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Monthly Archives: March 2016
What Are Smart Contracts? Cryptocurrency's Killer App …
Posted: March 4, 2016 at 11:45 am
This article contains interviews with Phil Raporport, drector of markets and trading at Ripple Labs, Stefan Thomas, CTO at Ripple Labs, and Chris Ellis, a cofounder of Feathercoin and show host with World Crypto Network.
What if you could cut your mortgage rate, make it easier to update your will, and ensure that your buddy was never able to weasel out of paying up on a bet? That and much more is the promise of smart contracts, a technology that is getting closer and closer to reality thanks to cryptocurrency.
Smart contracts are computer programs that can automatically execute the terms of a contract. Someday, these programs may replace lawyers and banks for handling certain common financial transactions.
And the potential for smart contracts goes way beyond simple transfers of funds. The door of a car or a house could be unlocked by connecting smart contracts to the Internet of everything. But as always with this cutting edge of financial technology, major questions abound: How will this all align with our current legal system? And, of course, will anyone actually use these things anyway?
The idea of smart contracts goes way back to 1994, nearly the dawn of the World Wide Web itself. That's when Nick Szabo, a cryptographer widely credited with laying the groundwork for bitcoin, first coined the term "smart contract." At core, these automated contracts work like any other computer program's if-then statements. They just happen to be doing it in a way that interacts with real-world assets. When a pre-programmed condition is triggered, the smart contract executes the corresponding contractual clause.
Szabo's original theories about how these contracts could work remained unrealized because there was no digitally native financial system that could support programmable transactions. (It defeats the purpose of smart contracts if a bank still has to manually authorize the release and transfer of money.) "One big hurdle to smart contracts is that computer programs can't really trigger payments right now," says Phil Rapoport, Ripple Labs' director of markets and trading.
The advent and increasingly widespread adoption of bitcoin is changing that, and as a result Szabo's idea has seen a revival. Smart contract technology is now being built on top of bitcoin and other virtual currencieswhat some have termed "Bitcoin 2.0" platforms. Because bitcoin is itself is a computer program, smart contracts can speak to it just like they would any other piece of code. The puzzle pieces are falling into place. A computer program can now trigger payments.
There are currently two major open source projects working on smart contracts, both of which have taken big leaps forward this year. One is called Codius and the other is Ethereum. Codius was developed by Ripple Labs, which also created its own digital currency called Ripple. Codius aims to be interoperable between a variety of cryptocurrency, such as Ripple and bitcoin, although it is managed by the private company.
"Codius can interact with other ledgers and web services. It can work on bitcoin and it can work on any other system," says Stefan Thomas, Ripple's CTO.
In contrast, Ethereum is an entirely new currency with smart contracts baked into its payment system. Originally developed by 20-year-old programmer Vitalik Buterin, it would replace other "coins" like bitcoin, but appears to be more of a community project.
Cryptocurrencies like bitcoin are poised to help smart contracts become reality. But the effect may also be reciprocal. Smart contracts can illustrate a unique benefit of virtual currencies that some advocates think could entice more users.
"Smart contracts are really the killer app of the cryptocurrency world," says Chris Ellis, host of a show about cryptocurrencies on the World Crypto Network.
Let's take a simple example, like a Super Bowl bet. Say you want to bet $500or roughly one bitcointhat the Patriots will win, while your friend is betting the same amount that the Packers will take the title. Step one is for you and your friend to place your bitcoin in a neutral account controlled by the smart contract. When the game is over and the smart contract is able to verify via ESPN, Reuters, or elsewhere that the Patriots beat the Packers, the smart contract would automatically deposit your bet and your winnings from your friend back into your account.
Because smart contracts are computer programs, it would be trivial to add more complex betting elements like odds and score differentials into the mix. While there are services out there today that might handle this sort of transaction, they all charge a fee. The key difference with smart contracts is that it is a decentralized system accessible to anyone, that doesn't require any intermediary party.
A more everyday example would be online shopping. "If you order something online you might not want to pay a merchant immediately until they fulfill their end of the bargain," says Rapoport. "So you could easily have a contract that looks for FedEx tracking data saying that the package you ordered has been delivered to your address before releasing payment to the sender."
If you think about a lot of routine financial transactions, what lawyers and banks do boils down to repetitively processing mundane tasks. And yet we still have to shell out huge fees for lawyers to go through wills or for banks to process our mortgage payments.
Smart contracts could automate and demystify these processes, making it so that ordinary people can save time and money.
Although you got your mortgage through a bank, that bank won't generally hold onto it for the entire 30-year loan; it will be sold to an investor. But you keep making payments to the bank, not the investor that owns your mortgage. The bank just becomes a processor for your monthly payments, sending a chunk to the investor, a slice to taxes, and a bit for homeowner's insurance.
"That's just a real simple operational task, but that bank will often take a quarter to a half percent per year to service that mortgage," says Rapoport. "They're just doing an operational headache of receiving payments and redirecting them. And they're charging people for that. But it's something that a smart contract could theoretically administer very easily."
If mortgage payments were handled by smart contracts, mortgage processing fees could be eliminated and that savings passed on to consumers. The result would be a lowered cost of home ownership.
Although smart contracts are still in their nascent stage, the potential is clear. If a simple enough user interface were developed it could remove a host of legal headaches, like updating your will. Imagine if allocating your assets after your death was as simple as moving an adjustable slider that determines who gets how much. Just like with the bet or FedEx example, once the smart contract can verify the triggering conditionin this case, your deaththe contract goes into effect and your assets are divvied up.
With all this, it may sound like we won't need lawyers anymore. But enthusiasts say that smart contracts should be seen as an evolution of the legal system, not its erasure.
"We don't think that this will replace the legal system as much as provide an intermediate layer between transacting and going to court," says Thomas.
Nonetheless, the role of lawyers might look very different in the future. Rather than having lawyers adjudicate individual contracts, the role of lawyers might shift to producing smart contract templates on a
competitive market. Contract selling points would be their quality, how customizable they are, and their ease of use. It sounds a bit like the marketplace for WordPress themes.
"I imagine a lot of people will create contracts that do different things," says Rapoport. "And they can essentially sell them for others to use. So if you make, for example, a really good equity agreement that has a bunch of different functionality a company can charge for access to their contract."
It's easy to think about a smart contract managing a will, up to a point. It all makes sense if you can imagine yourself keeping all of your assets in bitcoin. But what if you live in the real world and have physical possessions like, you know, most of us? The answer is something called smart property.
"This starts to get more sci-fi when we talk about smart property," says Ellis.
The so-called "Internet of Things" is constantly growing, with more and more interconnected devices out there every day. Some forward-thinking developers are already working on ways to combine the Internet of Things with bitcoin infrastructure so that something like a bitcoin can actually represent a physical object. That token is what these developers call smart property.
But more important than representing some object, these new smart property tokens would actually grant ownership and control to a networked object, whether that be a computer, a car, or even a house.
How does this all come together?
Ellis gives the example of renting out his house. "Let's say all the locks are Internet-enabled and they've all got network connections. When you make a bitcoin transaction for the rent, the smart contract you and I agreed to automatically unlocks the house for you. You just go in using keys stored on your smartphone."
A smart contract would also make it trivial to set up dates when those digital keys would automatically expire. It sounds a bit like Airbnb without the need for Airbnb.
And if you think about it, that's the fundamental transformation smart contracts are after. A service like Airbnb is desirable because it obviates the need for the host and the guest to trust each otherthey both only need to trust Airbnb. If the guest doesn't pay up, or the host doesn't leave the keys, either of them can take it up with Airbnb.
Doing the same sublet with a smart contract would supplant a business model like Airbnb's. The homeowner and renter still don't need to trust each otherthey just need to trust the smart contract. Smart contracts would decentralize the model of who needs to be trusted. And in doing so, it would cut out hefty fees by brokering services like Airbnb.
But smart contracts don't have to just disrupt existing business models. They can also complement them. Way back in his '94 essay, Nick Szabo envisioned the idea of smart property writing that "smart property might be created by embedding smart contracts in physical objects." His example of choice was a car loan, writing that if you miss a car payment, the smart contract could automatically revoke your digital keys to operate the car. No doubt car dealerships would find this appealing.
Admittedly, at some point it does start to sound like the makings of a dystopian sci-fi film. If you can't make a payment all of a sudden your car could be digitally and remotely repossessed, all without any human interaction.
But in theory, the upside is that financial institutions should be more willing to take risks on people who might not otherwise get loans. Because, worst case scenario, if someone can't pay up, it's inconsequential for the bank to take back the asset in question.
In addition to expanding opportunities to get credit, smart contracts also have the potential to open up access to the legal system for disadvantaged people who might not otherwise be able to reap its benefits. Thomas believes that smart contracts "will make the legal system available to people who might not be able to afford it on their own."
Although the law in theory treats everyone equally, you more often than not need money to take someone to court over a breach of contract.
"At present justice really only works if you can afford a lawyer to enforce that agreement. So once smart contracts have the ability to enforce agreements on their own it will be game-changing. " says Ellis.
Of course it may not play out that cleanly in reality. While this all sounds good and noble in theory, it's impossible to predict how a smart contract would hold up in court if it were ever challenged. Dethroning lawyers as the high priests of arbitrating contracts is certainly appealing. But do we run the risk of just replacing literacy in legalese with literacy in code?
Rapoport acknowledges that there may be drawbacks. "Everyone reads English, so in some ways it's easier to read a traditional contract. But this is still very bleeding-edge technology, so who knows what kinds of user-facing improvements will be made eventually?"
Despite unforeseen pitfalls, the promise of smart contracts is clear. Right now we're waiting to see if either Ethereum or Ripple's Codius will be able to become usable and really take off.
"Right now there are lot of clever people working on this who are high on ideas because they can see the potential," says Ellis "What we don't know yet is who is going to win this raceRipple or Ethereum. It's a bit like VHS vs. Betamax."
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What Are Smart Contracts? Cryptocurrency's Killer App ...
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What Are Smart Contracts? Cryptocurrency’s Killer App …
Posted: at 9:44 am
This article contains interviews with Phil Raporport, drector of markets and trading at Ripple Labs, Stefan Thomas, CTO at Ripple Labs, and Chris Ellis, a cofounder of Feathercoin and show host with World Crypto Network.
What if you could cut your mortgage rate, make it easier to update your will, and ensure that your buddy was never able to weasel out of paying up on a bet? That and much more is the promise of smart contracts, a technology that is getting closer and closer to reality thanks to cryptocurrency.
Smart contracts are computer programs that can automatically execute the terms of a contract. Someday, these programs may replace lawyers and banks for handling certain common financial transactions.
And the potential for smart contracts goes way beyond simple transfers of funds. The door of a car or a house could be unlocked by connecting smart contracts to the Internet of everything. But as always with this cutting edge of financial technology, major questions abound: How will this all align with our current legal system? And, of course, will anyone actually use these things anyway?
The idea of smart contracts goes way back to 1994, nearly the dawn of the World Wide Web itself. That's when Nick Szabo, a cryptographer widely credited with laying the groundwork for bitcoin, first coined the term "smart contract." At core, these automated contracts work like any other computer program's if-then statements. They just happen to be doing it in a way that interacts with real-world assets. When a pre-programmed condition is triggered, the smart contract executes the corresponding contractual clause.
Szabo's original theories about how these contracts could work remained unrealized because there was no digitally native financial system that could support programmable transactions. (It defeats the purpose of smart contracts if a bank still has to manually authorize the release and transfer of money.) "One big hurdle to smart contracts is that computer programs can't really trigger payments right now," says Phil Rapoport, Ripple Labs' director of markets and trading.
The advent and increasingly widespread adoption of bitcoin is changing that, and as a result Szabo's idea has seen a revival. Smart contract technology is now being built on top of bitcoin and other virtual currencieswhat some have termed "Bitcoin 2.0" platforms. Because bitcoin is itself is a computer program, smart contracts can speak to it just like they would any other piece of code. The puzzle pieces are falling into place. A computer program can now trigger payments.
There are currently two major open source projects working on smart contracts, both of which have taken big leaps forward this year. One is called Codius and the other is Ethereum. Codius was developed by Ripple Labs, which also created its own digital currency called Ripple. Codius aims to be interoperable between a variety of cryptocurrency, such as Ripple and bitcoin, although it is managed by the private company.
"Codius can interact with other ledgers and web services. It can work on bitcoin and it can work on any other system," says Stefan Thomas, Ripple's CTO.
In contrast, Ethereum is an entirely new currency with smart contracts baked into its payment system. Originally developed by 20-year-old programmer Vitalik Buterin, it would replace other "coins" like bitcoin, but appears to be more of a community project.
Cryptocurrencies like bitcoin are poised to help smart contracts become reality. But the effect may also be reciprocal. Smart contracts can illustrate a unique benefit of virtual currencies that some advocates think could entice more users.
"Smart contracts are really the killer app of the cryptocurrency world," says Chris Ellis, host of a show about cryptocurrencies on the World Crypto Network.
Let's take a simple example, like a Super Bowl bet. Say you want to bet $500or roughly one bitcointhat the Patriots will win, while your friend is betting the same amount that the Packers will take the title. Step one is for you and your friend to place your bitcoin in a neutral account controlled by the smart contract. When the game is over and the smart contract is able to verify via ESPN, Reuters, or elsewhere that the Patriots beat the Packers, the smart contract would automatically deposit your bet and your winnings from your friend back into your account.
Because smart contracts are computer programs, it would be trivial to add more complex betting elements like odds and score differentials into the mix. While there are services out there today that might handle this sort of transaction, they all charge a fee. The key difference with smart contracts is that it is a decentralized system accessible to anyone, that doesn't require any intermediary party.
A more everyday example would be online shopping. "If you order something online you might not want to pay a merchant immediately until they fulfill their end of the bargain," says Rapoport. "So you could easily have a contract that looks for FedEx tracking data saying that the package you ordered has been delivered to your address before releasing payment to the sender."
If you think about a lot of routine financial transactions, what lawyers and banks do boils down to repetitively processing mundane tasks. And yet we still have to shell out huge fees for lawyers to go through wills or for banks to process our mortgage payments.
Smart contracts could automate and demystify these processes, making it so that ordinary people can save time and money.
Although you got your mortgage through a bank, that bank won't generally hold onto it for the entire 30-year loan; it will be sold to an investor. But you keep making payments to the bank, not the investor that owns your mortgage. The bank just becomes a processor for your monthly payments, sending a chunk to the investor, a slice to taxes, and a bit for homeowner's insurance.
"That's just a real simple operational task, but that bank will often take a quarter to a half percent per year to service that mortgage," says Rapoport. "They're just doing an operational headache of receiving payments and redirecting them. And they're charging people for that. But it's something that a smart contract could theoretically administer very easily."
If mortgage payments were handled by smart contracts, mortgage processing fees could be eliminated and that savings passed on to consumers. The result would be a lowered cost of home ownership.
Although smart contracts are still in their nascent stage, the potential is clear. If a simple enough user interface were developed it could remove a host of legal headaches, like updating your will. Imagine if allocating your assets after your death was as simple as moving an adjustable slider that determines who gets how much. Just like with the bet or FedEx example, once the smart contract can verify the triggering conditionin this case, your deaththe contract goes into effect and your assets are divvied up.
With all this, it may sound like we won't need lawyers anymore. But enthusiasts say that smart contracts should be seen as an evolution of the legal system, not its erasure.
"We don't think that this will replace the legal system as much as provide an intermediate layer between transacting and going to court," says Thomas.
Nonetheless, the role of lawyers might look very different in the future. Rather than having lawyers adjudicate individual contracts, the role of lawyers might shift to producing smart contract templates on a competitive market. Contract selling points would be their quality, how customizable they are, and their ease of use. It sounds a bit like the marketplace for WordPress themes.
"I imagine a lot of people will create contracts that do different things," says Rapoport. "And they can essentially sell them for others to use. So if you make, for example, a really good equity agreement that has a bunch of different functionality a company can charge for access to their contract."
It's easy to think about a smart contract managing a will, up to a point. It all makes sense if you can imagine yourself keeping all of your assets in bitcoin. But what if you live in the real world and have physical possessions like, you know, most of us? The answer is something called smart property.
"This starts to get more sci-fi when we talk about smart property," says Ellis.
The so-called "Internet of Things" is constantly growing, with more and more interconnected devices out there every day. Some forward-thinking developers are already working on ways to combine the Internet of Things with bitcoin infrastructure so that something like a bitcoin can actually represent a physical object. That token is what these developers call smart property.
But more important than representing some object, these new smart property tokens would actually grant ownership and control to a networked object, whether that be a computer, a car, or even a house.
How does this all come together?
Ellis gives the example of renting out his house. "Let's say all the locks are Internet-enabled and they've all got network connections. When you make a bitcoin transaction for the rent, the smart contract you and I agreed to automatically unlocks the house for you. You just go in using keys stored on your smartphone."
A smart contract would also make it trivial to set up dates when those digital keys would automatically expire. It sounds a bit like Airbnb without the need for Airbnb.
And if you think about it, that's the fundamental transformation smart contracts are after. A service like Airbnb is desirable because it obviates the need for the host and the guest to trust each otherthey both only need to trust Airbnb. If the guest doesn't pay up, or the host doesn't leave the keys, either of them can take it up with Airbnb.
Doing the same sublet with a smart contract would supplant a business model like Airbnb's. The homeowner and renter still don't need to trust each otherthey just need to trust the smart contract. Smart contracts would decentralize the model of who needs to be trusted. And in doing so, it would cut out hefty fees by brokering services like Airbnb.
But smart contracts don't have to just disrupt existing business models. They can also complement them. Way back in his '94 essay, Nick Szabo envisioned the idea of smart property writing that "smart property might be created by embedding smart contracts in physical objects." His example of choice was a car loan, writing that if you miss a car payment, the smart contract could automatically revoke your digital keys to operate the car. No doubt car dealerships would find this appealing.
Admittedly, at some point it does start to sound like the makings of a dystopian sci-fi film. If you can't make a payment all of a sudden your car could be digitally and remotely repossessed, all without any human interaction.
But in theory, the upside is that financial institutions should be more willing to take risks on people who might not otherwise get loans. Because, worst case scenario, if someone can't pay up, it's inconsequential for the bank to take back the asset in question.
In addition to expanding opportunities to get credit, smart contracts also have the potential to open up access to the legal system for disadvantaged people who might not otherwise be able to reap its benefits. Thomas believes that smart contracts "will make the legal system available to people who might not be able to afford it on their own."
Although the law in theory treats everyone equally, you more often than not need money to take someone to court over a breach of contract.
"At present justice really only works if you can afford a lawyer to enforce that agreement. So once smart contracts have the ability to enforce agreements on their own it will be game-changing. " says Ellis.
Of course it may not play out that cleanly in reality. While this all sounds good and noble in theory, it's impossible to predict how a smart contract would hold up in court if it were ever challenged. Dethroning lawyers as the high priests of arbitrating contracts is certainly appealing. But do we run the risk of just replacing literacy in legalese with literacy in code?
Rapoport acknowledges that there may be drawbacks. "Everyone reads English, so in some ways it's easier to read a traditional contract. But this is still very bleeding-edge technology, so who knows what kinds of user-facing improvements will be made eventually?"
Despite unforeseen pitfalls, the promise of smart contracts is clear. Right now we're waiting to see if either Ethereum or Ripple's Codius will be able to become usable and really take off.
"Right now there are lot of clever people working on this who are high on ideas because they can see the potential," says Ellis "What we don't know yet is who is going to win this raceRipple or Ethereum. It's a bit like VHS vs. Betamax."
Excerpt from:
What Are Smart Contracts? Cryptocurrency's Killer App ...
Posted in Cryptocurrency
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DNA sequencing – Wikipedia, the free encyclopedia
Posted: March 3, 2016 at 4:42 pm
DNA sequencing is the process of determining the precise order of nucleotides within a DNA molecule. It includes any method or technology that is used to determine the order of the four basesadenine, guanine, cytosine, and thyminein a strand of DNA. The advent of rapid DNA sequencing methods has greatly accelerated biological and medical research and discovery.
Knowledge of DNA sequences has become indispensable for basic biological research, and in numerous applied fields such as medical diagnosis, biotechnology, forensic biology, virology and biological systematics. The rapid speed of sequencing attained with modern DNA sequencing technology has been instrumental in the sequencing of complete DNA sequences, or genomes of numerous types and species of life, including the human genome and other complete DNA sequences of many animal, plant, and microbial species.
The first DNA sequences were obtained in the early 1970s by academic researchers using laborious methods based on two-dimensional chromatography. Following the development of fluorescence-based sequencing methods with a DNA sequencer,[1] DNA sequencing has become easier and orders of magnitude faster.[2]
DNA sequencing may be used to determine the sequence of individual genes, larger genetic regions (i.e. clusters of genes or operons), full chromosomes or entire genomes. Sequencing provides the order of individual nucleotides present in molecules of DNA or RNA isolated from animals, plants, bacteria, archaea, or virtually any other source of genetic information. This information is useful to various fields of biology and other sciences, medicine, forensics, and other areas of study.
Sequencing is used in molecular biology to study genomes and the proteins they encode. Information obtained using sequencing allows researchers to identify changes in genes, associations with diseases and phenotypes, and identify potential drug targets.
Since DNA is an informative macromolecule in terms of transmission from one generation to another, DNA sequencing is used in evolutionary biology to study how different organisms are related and how they evolved.
The field of metagenomics involves identification of organisms present in a body of water, sewage, dirt, debris filtered from the air, or swab samples from organisms. Knowing which organisms are present in a particular environment is critical to research in ecology, epidemiology, microbiology, and other fields. Sequencing enables researchers to determine which types of microbes may be present in a microbiome, for example.
Medical technicians may sequence genes (or, theoretically, full genomes) from patients to determine if there is risk of genetic diseases. This is a form of genetic testing, though some genetic tests may not involve DNA sequencing.
DNA sequencing may be used along with DNA profiling methods for forensic identification and paternity testing.
The canonical structure of DNA has four bases: thymine (T), adenine (A), cytosine (C), and guanine (G). DNA sequencing is the determination of the physical order of these bases in a molecule of DNA. However, there are many other bases that may be present in a molecule. In some viruses (specifically, bacteriophage), cytosine may be replaced by hydroxy methyl or hydroxy methyl glucose cytosine.[3] In mammalian DNA, variant bases with methyl groups or phosphosulfate may be found.[4][5] Depending on the sequencing technique, a particular modification may or may not be detected, e.g., the 5mC (5 methyl cytosine) common in humans may or may not be detected.[6]
Deoxyribonucleic acid (DNA) was first discovered and isolated by Friedrich Miescher in 1869, but it remained understudied for many decades because proteins, rather than DNA, were thought to hold the genetic blueprint to life. This situation changed after 1944 as a result of some experiments by Oswald Avery, Colin MacLeod, and Maclyn McCarty demonstrated that purified DNA could change one strain of bacteria into another type. This was the first time that DNA was shown capable of transforming the properties of cells.
In 1953 James Watson and Francis Crick put forward their double-helix model of DNA which depicted DNA being made up of two strands of nucleotides coiled around each other, linked together by hydrogen bonds, in a spiral configuration. Each strand they argued was composed of four complementary nucleotides: adenine (A), cytosine (C), guanine (G) and thymine (T) and was oriented in opposite directions. Such a structure they proposed allowed each strand to reconstruct the other and was central to the passing on of hereditary information between generations.[7]
The foundation for sequencing DNA was first laid by the work of Fred Sanger who by 1955 had completed the sequence of all the amino acids in insulin, a small protein secreted by the pancreas. This provided the first conclusive evidence that proteins were chemical entities with a specific molecular pattern rather than a random mixture of material suspended in fluid. Sanger's success in sequencing insulin greatly electrified x-ray crystallographers, including Watson and Crick who by now were trying to understand how DNA directed the formation of proteins within a cell. Soon after attending a series of lectures given by Fred Sanger in October 1954, Crick began to develop a theory which argued that the arrangement of nucleotides in DNA determined the sequence of amino acids in proteins which in turn helped determine the function of a protein. He published this theory in 1958.[8]
RNA sequencing was one of the earliest forms of nucleotide sequencing. The major landmark of RNA sequencing is the sequence of the first complete gene and the complete genome of Bacteriophage MS2, identified and published by Walter Fiers and his coworkers at the University of Ghent (Ghent, Belgium), in 1972[9] and 1976.[10]
The first method for determining DNA sequences involved a location-specific primer extension strategy established by Ray Wu at Cornell University in 1970.[11] DNA polymerase catalysis and specific nucleotide labeling, both of which figure prominently in current sequencing schemes, were used to sequence the cohesive ends of lambda phage DNA.[12][13][14] Between 1970 and 1973, Wu, R Padmanabhan and colleagues demonstrated that this method can be employed to determine any DNA sequence using synthetic location-specific primers.[15][16][17]Frederick Sanger then adopted this primer-extension strategy to develop more rapid DNA sequencing methods at the MRC Centre, Cambridge, UK and published a method for "DNA sequencing with chain-terminating inhibitors" in 1977.[18]Walter Gilbert and Allan Maxam at Harvard also developed sequencing methods, including one for "DNA sequencing by chemical degradation".[19][20] In 1973, Gilbert and Maxam reported the sequence of 24 basepairs using a method known as wandering-spot analysis.[21] Advancements in sequencing were aided by the concurrent development of recombinant DNA technology, allowing DNA samples to be isolated from sources other than viruses.
The first full DNA genome to be sequenced was that of bacteriophage X174 in 1977.[22]Medical Research Council scientists deciphered the complete DNA sequence of the Epstein-Barr virus in 1984, finding it contained 172,282 nucleotides. Completion of the sequence marked a significant turning point in DNA sequencing because it was achieved with no prior genetic profile knowledge of the virus.[23]
A non-radioactive method for transferring the DNA molecules of sequencing reaction mixtures onto an immobilizing matrix during electrophoresis was developed by Pohl and co-workers in the early 1980s.[24][25] Followed by the commercialization of the DNA sequencer "Direct-Blotting-Electrophoresis-System GATC 1500" by GATC Biotech, which was intensively used in the framework of the EU genome-sequencing programme, the complete DNA sequence of the yeast Saccharomyces cerevisiae chromosome II.[26]Leroy E. Hood's laboratory at the California Institute of Technology announced the first semi-automated DNA sequencing machine in 1986.[27] This was followed by Applied Biosystems' marketing of the first fully automated sequencing machine, the ABI 370, in 1987 and by Dupont's Genesis 2000[28] which used a novel fluorescent labeling technique enabling all four dideoxynucleotides to be identified in a single lane. By 1990, the U.S. National Institutes of Health (NIH) had begun large-scale sequencing trials on Mycoplasma capricolum, Escherichia coli, Caenorhabditis elegans, and Saccharomyces cerevisiae at a cost of US$0.75 per base. Meanwhile, sequencing of human cDNA sequences called expressed sequence tags began in Craig Venter's lab, an attempt to capture the coding fraction of the human genome.[29] In 1995, Venter, Hamilton Smith, and colleagues at The Institute for Genomic Research (TIGR) published the first complete genome of a free-living organism, the bacterium Haemophilus influenzae. The circular chromosome contains 1,830,137 bases and its publication in the journal Science[30] marked the first published use of whole-genome shotgun sequencing, eliminating the need for initial mapping efforts.
By 2001, shotgun sequencing methods had been used to produce a draft sequence of the human genome.[31][32]
Several new methods for DNA sequencing were developed in the mid to late 1990s and were implemented in commercial DNA sequencers by the year 2000.
On October 26, 1990, Roger Tsien, Pepi Ross, Margaret Fahnestock and Allan J Johnston filed a patent describing stepwise ("base-by-base") sequencing with removable 3' blockers on DNA arrays (blots and single DNA molecules).[33] In 1996, Pl Nyrn and his student Mostafa Ronaghi at the Royal Institute of Technology in Stockholm published their method of pyrosequencing.[34]
On April 1, 1997, Pascal Mayer and Laurent Farinelli submitted patents to the World Intellectual Property Organization describing DNA colony sequencing.[35] The DNA sample preparation and random surface-PCR arraying methods described in this patent, coupled to Roger Tsien et al.'s "base-by-base" sequencing method, is now implemented in Illumina's Hi-Seq genome sequencers.
Lynx Therapeutics published and marketed "Massively parallel signature sequencing", or MPSS, in 2000. This method incorporated a parallelized, adapter/ligation-mediated, bead-based sequencing technology and served as the first commercially available "next-generation" sequencing method, though no DNA sequencers were sold to independent laboratories.[36]
In 2004, 454 Life Sciences marketed a parallelized version of pyrosequencing.[37] The first version of their machine reduced sequencing costs 6-fold compared to automated Sanger sequencing, and was the second of the new generation of sequencing technologies, after MPSS.[38]
The large quantities of data produced by DNA sequencing have also required development of new methods and programs for sequence analysis. Phil Green and Brent Ewing of the University of Washington described their phred quality score for sequencer data analysis in 1998.[39]
Allan Maxam and Walter Gilbert published a DNA sequencing method in 1977 based on chemical modification of DNA and subsequent cleavage at specific bases.[19] Also known as chemical sequencing, this method allowed purified samples of double-stranded DNA to be used without further cloning. This method's use of radioactive labeling and its technical complexity discouraged extensive use after refinements in the Sanger methods had been made.
Maxam-Gilbert sequencing requires radioactive labeling at one 5' end of the DNA and purification of the DNA fragment to be sequenced. Chemical treatment then generates breaks at a small proportion of one or two of the four nucleotide bases in each of four reactions (G, A+G, C, C+T). The concentration of the modifying chemicals is controlled to introduce on average one modification per DNA molecule. Thus a series of labeled fragments is generated, from the radiolabeled end to the first "cut" site in each molecule. The fragments in the four reactions are electrophoresed side by side in denaturing acrylamide gels for size separation. To visualize the fragments, the gel is exposed to X-ray film for autoradiography, yielding a series of dark bands each corresponding to a radiolabeled DNA fragment, from which the sequence may be inferred.[19]
The chain-termination method developed by Frederick Sanger and coworkers in 1977 soon became the method of choice, owing to its relative ease and reliability.[18][40] When invented, the chain-terminator method used fewer toxic chemicals and lower amounts of radioactivity than the Maxam and Gilbert method. Because of its comparative ease, the Sanger method was soon automated and was the method used in the first generation of DNA sequencers.
Sanger sequencing is the method which prevailed from the 1980s until the mid-2000s. Over that period, great advances were made in the technique, such as fluorescent labelling, capillary electrophoresis, and general automation. These developments allowed much more efficient sequencing, leading to lower costs. The Sanger method, in mass production form, is the technology which produced the first human genome in 2001, ushering in the age of genomics. However, later in the decade, radically different approaches reached the market, bringing the cost per genome down from $100 million in 2001 to $10,000 in 2011.[41]
Large-scale sequencing often aims at sequencing very long DNA pieces, such as whole chromosomes, although large-scale sequencing can also be used to generate very large numbers of short sequences, such as found in phage display. For longer targets such as chromosomes, common approaches consist of cutting (with restriction enzymes) or shearing (with mechanical forces) large DNA fragments into shorter DNA fragments. The fragmented DNA may then be cloned into a DNA vector and amplified in a bacterial host such as Escherichia coli. Short DNA fragments purified from individual bacterial colonies are individually sequenced and assembled electronically into one long, contiguous sequence. Studies have shown that adding a size selection step to collect DNA fragments of uniform size can improve sequencing efficiency and accuracy of the genome assembly. In these studies, automated sizing has proven to be more reproducible and precise than manual gel sizing.[42][43][44]
The term "de novo sequencing" specifically refers to methods used to determine the sequence of DNA with no previously known sequence. De novo translates from Latin as "from the beginning". Gaps in the assembled sequence may be filled by primer walking. The different strategies have different tradeoffs in speed and accuracy; shotgun methods are often used for sequencing large genomes, but its assembly is complex and difficult, particularly with sequence repeats often causing gaps in genome assembly.
Most sequencing approaches use an in vitro cloning step to amplify individual DNA molecules, because their molecular detection methods are not sensitive enough for single molecule sequencing. Emulsion PCR[45] isolates individual DNA molecules along with primer-coated beads in aqueous droplets within an oil phase. A polymerase chain reaction (PCR) then coats each bead with clonal copies of the DNA molecule followed by immobilization for later sequencing. Emulsion PCR is used in the methods developed by Marguilis et al. (commercialized by 454 Life Sciences), Shendure and Porreca et al. (also known as "Polony sequencing") and SOLiD sequencing, (developed by Agencourt, later Applied Biosystems, now Life Technologies).[46][47][48]
Shotgun sequencing is a sequencing method designed for analysis of DNA sequences longer than 1000 base pairs, up to and including entire chromosomes. This method requires the target DNA to be broken into random fragments. After sequencing individual fragments, the sequences can be reassembled on the basis of their overlapping regions.[49]
Another method for in vitro clonal amplification is bridge PCR, in which fragments are amplified upon primers attached to a solid surface[35][50][51] and form "DNA colonies" or "DNA clusters". This method is used in the Illumina Genome Analyzer sequencers. Single-molecule methods, such as that developed by Stephen Quake's laboratory (later commercialized by Helicos) are an exception: they use bright fluorophores and laser excitation to detect base addition events from individual DNA molecules fixed to a surface, eliminating the need for molecular amplification.[52]
Next-generation sequencing applies to genome sequencing, genome resequencing, transcriptome profiling (RNA-Seq), DNA-protein interactions (ChIP-sequencing), and epigenome characterization.[53] Resequencing is necessary, because the genome of a single individual of a species will not indicate all of the genome variations among other individuals of the same species.
The high demand for low-cost sequencing has driven the development of high-throughput sequencing (or next-generation sequencing) technologies that parallelize the sequencing process, producing thousands or millions of sequences concurrently.[54][55] High-throughput sequencing technologies are intended to lower the cost of DNA sequencing beyond what is possible with standard dye-terminator methods.[38] In ultra-high-throughput sequencing as many as 500,000 sequencing-by-synthesis operations may be run in parallel.[56][57][58]
The first of the next-generation sequencing technologies, massively parallel signature sequencing (or MPSS), was developed in the 1990s at Lynx Therapeutics, a company founded in 1992 by Sydney Brenner and Sam Eletr. MPSS was a bead-based method that used a complex approach of adapter ligation followed by adapter decoding, reading the sequence in increments of four nucleotides. This method made it susceptible to sequence-specific bias or loss of specific sequences. Because the technology was so complex, MPSS was only performed 'in-house' by Lynx Therapeutics and no DNA sequencing machines were sold to independent laboratories. Lynx Therapeutics merged with Solexa (later acquired by Illumina) in 2004, leading to the development of sequencing-by-synthesis, a simpler approach acquired from Manteia Predictive Medicine, which rendered MPSS obsolete. However, the essential properties of the MPSS output were typical of later "next-generation" data types, including hundreds of thousands of short DNA sequences. In the case of MPSS, these were typically used for sequencing cDNA for measurements of gene expression levels.[36]
The Polony sequencing method, developed in the laboratory of George M. Church at Harvard, was among the first next-generation sequencing systems and was used to sequence a full E. coli genome in 2005.[71] It combined an in vitro paired-tag library with emulsion PCR, an automated microscope, and ligation-based sequencing chemistry to sequence an E. coli genome at an accuracy of >99.9999% and a cost approximately 1/9 that of Sanger sequencing.[71] The technology was licensed to Agencourt Biosciences, subsequently spun out into Agencourt Personal Genomics, and eventually incorporated into the Applied Biosystems SOLiD platform. Applied Biosystems was later acquired by Life Technologies, now part of Thermo Fisher Scientific.
A parallelized version of pyrosequencing was developed by 454 Life Sciences, which has since been acquired by Roche Diagnostics. The method amplifies DNA inside water droplets in an oil solution (emulsion PCR), with each droplet containing a single DNA template attached to a single primer-coated bead that then forms a clonal colony. The sequencing machine contains many picoliter-volume wells each containing a single bead and sequencing enzymes. Pyrosequencing uses luciferase to generate light for detection of the individual nucleotides added to the nascent DNA, and the combined data are used to generate sequence read-outs.[46] This technology provides intermediate read length and price per base compared to Sanger sequencing on one end and Solexa and SOLiD on the other.[38]
Solexa, now part of Illumina, was founded by Shankar Balasubramanian and David Klenerman in 1998, and developed a sequencing method based on reversible dye-terminators technology, and engineered polymerases.[72] The terminated chemistry was developed internally at Solexa and the concept of the Solexa system was invented by Balasubramanian and Klenerman from Cambridge University's chemistry department. In 2004, Solexa acquired the company Manteia Predictive Medicine in order to gain a massivelly parallel sequencing technology invented in 1997 by Pascal Mayer and Laurent Farinelli.[35] It is based on "DNA Clusters" or "DNA colonies", which involves the clonal amplification of DNA on a surface. The cluster technology was co-acquired with Lynx Therapeutics of California. Solexa Ltd. later merged with Lynx to form Solexa Inc.
In this method, DNA molecules and primers are first attached on a slide or flow cell and amplified with polymerase so that local clonal DNA colonies, later coined "DNA clusters", are formed. To determine the sequence, four types of reversible terminator bases (RT-bases) are added and non-incorporated nucleotides are washed away. A camera takes images of the fluorescently labeled nucleotides. Then the dye, along with the terminal 3' blocker, is chemically removed from the DNA, allowing for the next cycle to begin. Unlike pyrosequencing, the DNA chains are extended one nucleotide at a time and image acquisition can be performed at a delayed moment, allowing for very large arrays of DNA colonies to be captured by sequential images taken from a single camera.
Decoupling the enzymatic reaction and the image capture allows for optimal throughput and theoretically unlimited sequencing capacity. With an optimal configuration, the ultimately reachable instrument throughput is thus dictated solely by the analog-to-digital conversion rate of the camera, multiplied by the number of cameras and divided by the number of pixels per DNA colony required for visualizing them optimally (approximately 10 pixels/colony). In 2012, with cameras operating at more than 10MHz A/D conversion rates and available optics, fluidics and enzymatics, throughput can be multiples of 1 million nucleotides/second, corresponding roughly to 1 human genome equivalent at 1x coverage per hour per instrument, and 1 human genome re-sequenced (at approx. 30x) per day per instrument (equipped with a single camera).[73]
Applied Biosystems' (now a Life Technologies brand) SOLiD technology employs sequencing by ligation. Here, a pool of all possible oligonucleotides of a fixed length are labeled according to the sequenced position. Oligonucleotides are annealed and ligated; the preferential ligation by DNA ligase for matching sequences results in a signal informative of the nucleotide at that position. Before sequencing, the DNA is amplified by emulsion PCR. The resulting beads, each containing single copies of the same DNA molecule, are deposited on a glass slide.[74] The result is sequences of quantities and lengths comparable to Illumina sequencing.[38] This sequencing by ligation method has been reported to have some issue sequencing palindromic sequences.[70]
Ion Torrent Systems Inc. (now owned by Life Technologies) developed a system based on using standard sequencing chemistry, but with a novel, semiconductor based detection system. This method of sequencing is based on the detection of hydrogen ions that are released during the polymerisation of DNA, as opposed to the optical methods used in other sequencing systems. A microwell containing a template DNA strand to be sequenced is flooded with a single type of nucleotide. If the introduced nucleotide is complementary to the leading template nucleotide it is incorporated into the growing complementary strand. This causes the release of a hydrogen ion that triggers a hypersensitive ion sensor, which indicates that a reaction has occurred. If homopolymer repeats are present in the template sequence multiple nucleotides will be incorporated in a single cycle. This leads to a corresponding number of released hydrogens and a proportionally higher electronic signal.[75]
DNA nanoball sequencing is a type of high throughput sequencing technology used to determine the entire genomic sequence of an organism. The company Complete Genomics uses this technology to sequence samples submitted by independent researchers. The method uses rolling circle replication to amplify small fragments of genomic DNA into DNA nanoballs. Unchained sequencing by ligation is then used to determine the nucleotide sequence.[76] This method of DNA sequencing allows large numbers of DNA nanoballs to be sequenced per run and at low reagent costs compared to other next generation sequencing platforms.[77] However, only short sequences of DNA are determined from each DNA nanoball which makes mapping the short reads to a reference genome difficult.[76] This technology has been used for multiple genome sequencing projects and is scheduled to be used for more.[78]
Heliscope sequencing is a method of single-molecule sequencing developed by Helicos Biosciences. It uses DNA fragments with added poly-A tail adapters which are attached to the flow cell surface. The next steps involve extension-based sequencing with cyclic washes of the flow cell with fluorescently labeled nucleotides (one nucleotide type at a time, as with the Sanger method). The reads are performed by the Heliscope sequencer.[79][80] The reads are short, averaging 35 bp.[81] In 2009 a human genome was sequenced using the Heliscope, however in 2012 the company went bankrupt.[82]
SMRT sequencing is based on the sequencing by synthesis approach. The DNA is synthesized in zero-mode wave-guides (ZMWs) small well-like containers with the capturing tools located at the bottom of the well. The sequencing is performed with use of unmodified polymerase (attached to the ZMW bottom) and fluorescently labelled nucleotides flowing freely in the solution. The wells are constructed in a way that only the fluorescence occurring by the bottom of the well is detected. The fluorescent label is detached from the nucleotide upon its incorporation into the DNA strand, leaving an unmodified DNA strand. According to Pacific Biosciences (PacBio), the SMRT technology developer, this methodology allows detection of nucleotide modifications (such as cytosine methylation). This happens through the observation of polymerase kinetics. This approach allows reads of 20,000 nucleotides or more, with average read lengths of 5 kilobases.[65][83] In 2015, Pacific Biosciences announced the launch of a new sequencing instrument called the Sequel System, with 1 million ZMWs compared to 150,000 ZMWs in the PacBio RS II instrument.[84][85]
DNA sequencing methods currently under development include reading the sequence as a DNA strand transits through nanopores,[86][87] and microscopy-based techniques, such as atomic force microscopy or transmission electron microscopy that are used to identify the positions of individual nucleotides within long DNA fragments (>5,000 bp) by nucleotide labeling with heavier elements (e.g., halogens) for visual detection and recording.[88][89] Third generation technologies aim to increase throughput and decrease the time to result and cost by eliminating the need for excessive reagents and harnessing the processivity of DNA polymerase.[90]
This method is based on the readout of electrical signals occurring at nucleotides passing by alpha-hemolysin pores covalently bound with cyclodextrin. The DNA passing through the nanopore changes its ion current. This change is dependent on the shape, size and length of the DNA sequence. Each type of the nucleotide blocks the ion flow through the pore for a different period of time. The method has a potential of development as it does not require modified nucleotides, however single nucleotide resolution is not yet available.[91]
Two main areas of nanopore sequencing in development are solid state nanopore sequencing, and protein based nanopore sequencing. Protein nanopore sequencing utilizes membrane protein complexes -Hemolysin and MspA (Mycobacterium Smegmatis Porin A), which show great promise given their ability to distinguish between individual and groups of nucleotides.[92] In contrast, solid-state nanopore sequencing utilizes synthetic materials such as silicon nitride and aluminum oxide and it is preferred for its superior mechanical ability and thermal and chemical stability.[93] The fabrication method is essential for this type of sequencing given that the nanopore array can contain hundreds of pores with diameters smaller than eight nanometers.[92]
The concept originated from the idea that single stranded DNA or RNA molecules can be electrophoretically driven in a strict linear sequence through a biological pore that can be less than eight nanometers, and can be detected given that the molecules release an ionic current while moving through the pore. The pore contains a detection region capable of recognizing different bases, with each base generating various time specific signals corresponding to the sequence of bases as they cross the pore which are then evaluated.[93] When implementing this process it is important to note that precise control over the DNA transport through the pore is crucial for success. Various enzymes such as exonucleases and polymerases have been used to moderate this process by positioning them near the pores entrance.[94]
Oxford Nanopore Technologies, a United Kingdom-based startup company, is currently developing products using nanopore sequencing. These products include the MinION, a handheld sequencer capable of generating more than 150 megabases of sequencing data in one run. The MinION is not yet available to the public and has been found to produce numerous errors, though further study may alleviate the issue.[95][96]
Another approach uses measurements of the electrical tunnelling currents across single-strand DNA as it moves through a channel. Depending on its electronic structure, each base affects the tunnelling current differently, allowing differentiation between different bases.[97]
The use of tunnelling currents has the potential to sequence orders of magnitude faster than ionic current methods and the sequencing of several DNA oligomers and micro-RNA has already been achieved.[98]
Sequencing by hybridization is a non-enzymatic method that uses a DNA microarray. A single pool of DNA whose sequence is to be determined is fluorescently labeled and hybridized to an array containing known sequences. Strong hybridization signals from a given spot on the array identifies its sequence in the DNA being sequenced.[99]
This method of sequencing utilizes binding characteristics of a library of short single stranded DNA molecules (oligonucleotides), also called DNA probes, to reconstruct a target DNA sequence. Non-specific hybrids are removed by washing and the target DNA is eluted.[100] Hybrids are re-arranged such that the DNA sequence can be reconstructed. The benefit of this sequencing type is its ability to capture a large number of targets with a homogenous coverage.[101] A large number of chemicals and starting DNA is usually required. However, with the advent of solution-based hybridization, much less equipment and chemicals are necessary.[100]
Mass spectrometry may be used to determine DNA sequences. Matrix-assisted laser desorption ionization time-of-flight mass spectrometry, or MALDI-TOF MS, has specifically been investigated as an alternative method to gel electrophoresis for visualizing DNA fragments. With this method, DNA fragments generated by chain-termination sequencing reactions are compared by mass rather than by size. The mass of each nucleotide is different from the others and this difference is detectable by mass spectrometry. Single-nucleotide mutations in a fragment can be more easily detected with MS than by gel electrophoresis alone. MALDI-TOF MS can more easily detect differences between RNA fragments, so researchers may indirectly sequence DNA with MS-based methods by converting it to RNA first.[102]
The higher resolution of DNA fragments permitted by MS-based methods is of special interest to researchers in forensic science, as they may wish to find single-nucleotide polymorphisms in human DNA samples to identify individuals. These samples may be highly degraded so forensic researchers often prefer mitochondrial DNA for its higher stability and applications for lineage studies. MS-based sequencing methods have been used to compare the sequences of human mitochondrial DNA from samples in a Federal Bureau of Investigation database[103] and from bones found in mass graves of World War I soldiers.[104]
Early chain-termination and TOF MS methods demonstrated read lengths of up to 100 base pairs.[105] Researchers have been unable to exceed this average read size; like chain-termination sequencing alone, MS-based DNA sequencing may not be suitable for large de novo sequencing projects. Even so, a recent study did use the short sequence reads and mass spectroscopy to compare single-nucleotide polymorphisms in pathogenic Streptococcus strains.[106]
In microfluidic Sanger sequencing the entire thermocycling amplification of DNA fragments as well as their separation by electrophoresis is done on a single glass wafer (approximately 10cm in diameter) thus reducing the reagent usage as well as cost.[107] In some instances researchers have shown that they can increase the throughput of conventional sequencing through the use of microchips.[108] Research will still need to be done in order to make this use of technology effective.
This approach directly visualizes the sequence of DNA molecules using electron microscopy. The first identification of DNA base pairs within intact DNA molecules by enzymatically incorporating modified bases, which contain atoms of increased atomic number, direct visualization and identification of individually labeled bases within a synthetic 3,272 base-pair DNA molecule and a 7,249 base-pair viral genome has been demonstrated.[109]
This method is based on use of RNA polymerase (RNAP), which is attached to a polystyrene bead. One end of DNA to be sequenced is attached to another bead, with both beads being placed in optical traps. RNAP motion during transcription brings the beads in closer and their relative distance changes, which can then be recorded at a single nucleotide resolution. The sequence is deduced based on the four readouts with lowered concentrations of each of the four nucleotide types, similarly to the Sanger method.[110] A comparison is made between regions and sequence information is deduced by comparing the known sequence regions to the unknown sequence regions.[111]
A method has been developed to analyze full sets of protein interactions using a combination of 454 pyrosequencing and an in vitro virus mRNA display method. Specifically, this method covalently links proteins of interest to the mRNAs encoding them, then detects the mRNA pieces using reverse transcription PCRs. The mRNA may then be amplified and sequenced. The combined method was titled IVV-HiTSeq and can be performed under cell-free conditions, though its results may not be representative of in vivo conditions.[112]
The success of a DNA sequencing protocol is dependent on the sample preparation. A successful DNA extraction will yield a sample with long, non-degraded strands of DNA which require further preparation according to the sequencing technology to be used. For Sanger sequencing, either cloning procedures or PCR are required prior to sequencing. In the case of next generation sequencing methods, library preparation is required before processing.[113]
With the advent of next generation sequencing, Illumina and Roche 454 methods have become a common approach to transcriptomic studies (RNAseq). RNA can be extracted from tissues of interest and converted to complimentary DNA (cDNA) using reverse transcriptasea DNA polymerase that synthesizes a complimentary DNA based on existing strands of RNA in a PCR-like manner.[114] Complimentary DNA can be processed the same way as genomic DNA, allowing the expression levels of RNAs to be determined for the tissue selected.[115]
In October 2006, the X Prize Foundation established an initiative to promote the development of full genome sequencing technologies, called the Archon X Prize, intending to award $10 million to "the first Team that can build a device and use it to sequence 100 human genomes within 10 days or less, with an accuracy of no more than one error in every 100,000 bases sequenced, with sequences accurately covering at least 98% of the genome, and at a recurring cost of no more than $10,000 (US) per genome."[116]
Each year the National Human Genome Research Institute, or NHGRI, promotes grants for new research and developments in genomics. 2010 grants and 2011 candidates include continuing work in microfluidic, polony and base-heavy sequencing methodologies.[117]
The sequencing technologies described here produce raw data that needs to be assembled into longer sequences such as complete genomes (sequence assembly). There are many computational challenges to achieve this, such as the evaluation of the raw sequence data which is done by programs and algorithms such as Phred and Phrap. Other challenges have to deal with repetitive sequences that often prevent complete genome assemblies because they occur in many places of the genome. As a consequence, many sequences may not be assigned to particular chromosomes. The production of raw sequence data is only the beginning of its detailed bioinformatical analysis.[118] Yet new methods for sequencing and correcting sequencing errors were developed.[119]
Sometimes, the raw reads produced by the sequencer are correct and precise only in a fraction of their length. Using the entire read may introduce artifacts in the downstream analyses like genome assembly, snp calling, or gene expression estimation. Two classes of trimming programs have been introduced, based on the window-based or the running-sum classes of algorithms.[120] This is a partial list of the trimming algorithms currently available, specifying the algorithm class they belong to:
Human genetics have been included within the field of bioethics since the early 1970s[127] and the growth in the use of DNA sequencing (particularly high-throughput sequencing) has introduced a number of ethical issues. One key issue is the ownership of an individual's DNA and the data produced when that DNA is sequenced.[128] Regarding the DNA molecule itself, the leading legal case on this topic, Moore v. Regents of the University of California (1990) ruled that individuals have no property rights to discarded cells or any profits made using these cells (for instance, as a patented cell line). However, individuals have a right to informed consent regarding removal and use of cells. Regarding the data produced through DNA sequencing, Moore gives the individual no rights to the information derived from their DNA.[128]
As DNA sequencing becomes more widespread, the storage, security and sharing of genomic data has also become more important.[128][129] For instance, one concern is that insurers may use an individual's genomic data to modify their quote, depending on the perceived future health of the individual based on their DNA.[129][130] In May 2008, the Genetic Information Nondiscrimination Act (GINA) was signed in the United States, prohibiting discrimination on the basis of genetic information with respect to health insurance and employment.[131][132] In 2012, the US Presidential Commission for the Study of Bioethical Issues reported that existing privacy legislation for DNA sequencing data such as GINA and the Health Insurance Portability and Accountability Act were insufficient, noting that whole-genome sequencing data was particularly sensitive, as it could be used to identify not only the individual from which the data was created, but also their relatives.[133][134]
Ethical issues have also been raised by the increasing use of genetic variation screening, both in newborns, and in adults by companies such as 23andMe.[135][136] It has been asserted that screening for genetic variations can be harmful, increasing anxiety in individuals who have been found to have an increased risk of disease.[137] For example, in one case noted in Time, doctors screening an ill baby for genetic variants chose not to inform the parents of an unrelated variant linked to dementia due to the harm it would cause to the parents.[138] However, a 2011 study in The New England Journal of Medicine has shown that individuals undergoing disease risk profiling did not show increased levels of anxiety.[137]
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Eugenics … death of the defenceless – creation.com
Posted: at 11:43 am
The legacy of Darwins cousin Galton
By Russell Grigg
Few ideas have done more harm to the human race in the last 120 years than those of Sir Francis Galton. He founded the evolutionary pseudo-science of eugenics. Today, ethnic cleansing, the use of abortion to eliminate defective unborn babies, infanticide, euthanasia, and the harvesting of unborn babies for research purposes all have a common foundation in the survival-of-the-fittest theory of eugenics. So who was Galton, what is eugenics, and how has it harmed humanity?
Photos Darwin by TFE Graphics, Hitler and Galton by Wikipedia.org
Francis Galton (featured on right in photo montage, right) was born into a Quaker family in Birmingham, England, in 1822. A grandson of Erasmus Darwin on his mothers side and so a cousin of Charles Darwin (pictured above left), he shared the Darwinian agnosticism and antagonism to Christianity for most of his adult life.
As a child, he had learned the alphabet by 18 months, was reading by age 2, memorizing poetry by five, and discussing the Iliad at six.1 In 1840, he began studies at Cambridge University in medicine and then in mathematics, but, due to a nervous breakdown, succeeded in gaining only a modest B.A. degree, in January 1844.2 When his father died that same year, he inherited such a fortune that he never again needed to work for a living.
This gave the wealthy young Galton free time not only for amusement, but also to dabble in a number of fields, including exploration of large areas of South West Africa, his reports of which gained him membership of the Royal Geographic Society in 1853, and three years later of the Royal Society. In that year, Galton married Louisa Butler, whose father had been Headmaster at Harrow School.
As an amateur scientist of boundless curiosity and energy, he went on to write some 14 books and over 200 papers.3 His inventions included the silent dog whistle, a teletype printer; and various instruments and techniques for measuring human intelligence and body parts; and he invented the weather map and discovered the existence of anticyclones.
The publication of Darwins Origin of Species in 1859 was undoubtedly a turning point in Galtons life. In 1869 he wrote to Darwin, [T]he appearance of your Origin of Species formed a real crisis in my life; your book drove away the constraint of my old superstition [i.e. religious arguments based on design] as if it had been a nightmare and was the first to give me freedom of thought.4
From Nott, J.C. and Gliddon, G.R., Indigenous Races of the Earth, J.B. Libbincott, Philadelphia, USA, 1868.
An allegedly scientific illustration from 1868 showing that blacks were less evolved than whites by suggesting similarities with a chimpanzee.
Even the famous evolutionist Stephen Jay Gould commented that the chimpanzee skull is falsely enlarged and the negro jaw falsely extended to suggest that negros rank even lower than apes. This demonstration was not from racist or fringe literature but from one of the leading scientific textbooks of its time. Todays militant evolutionists like to conveniently evade the social implications of their ideas, but history demonstrates otherwise.
Galton was among the first to recognize the implications for mankind of Darwins theory of evolution.5 He believed that talent, character, intellect, etc. were all inherited from ones ancestors, as was also any lack of these qualities. Thus the poor were not hapless victims of their circumstances, but were paupers because they were biologically inferior. This was contrary to the prevailing scientific view that all such qualities were due to environment, i.e. how and where a person was brought up.6 Galton believed that humans, like animals, could and should be selectively bred. In 1883, he coined the term eugenics [Greek: (eu) meaning well and (genos) meaning kind or offspring] for the study of ways of improving the physical and mental characteristics of the human race.
Galtons views left no room for the existence of a human soul, the grace of God in the human heart, human freedom to choose to be different, or even for the dignity of the individual. In his first published article on this subject, in 1865,7 He denied that mans rational faculties are a gift to him from God; he denied that mankind has been cursed with sinfulness since the day of Adam and Eve; and he viewed religious sentiments as nothing more than evolutionary devices to insure the survival of the human species.8
Concerning the sense of original sin, he wrote that [this] would show, according to my theory, not that man was fallen from a high estate, but that he was rapidly rising from a low one and that after myriads of years of barbarism, our race has but very recently grown to be civilized and religious.9
In Hereditary Genius (1869), Galton enlarged on all these ideas and proposed that a system of arranged marriages between men of distinction and women of wealth would eventually produce a gifted race. When Charles Darwin read this book, he wrote to Galton, You have made a convert of an opponent in one sense for I have always maintained that, excepting fools, men did not differ much in intellect, only in zeal and hard work .5 Galtons ideas undoubtedly helped him extend his evolution theory to man. Darwin did not mention Galton in his Origin, but referred to him no less than 11 times in his Descent of Man (1871).
Three International Eugenics Congresses were held in 1912, 1921 and 1932, with eugenics activists attending from Britain, the USA, Germany, France, Australia, Canada, India, Japan, Mauritius, Kenya and South Africa. Notables who supported the ideas preWorld War II included Winston Churchill, economist John Maynard Keynes, science fiction writer H.G. Wells10 and US Presidents Theodore Roosevelt and Calvin Coolidge. Galton received the Huxley Medal from the Anthropological Institute in 1901, the Darwin Medal from the Royal Society in 1902, the DarwinWallace Medal from the Linnean Society in 1908, and honorary degrees from Cambridge and Oxford Universities; he was knighted in 1909. Despite these honours, in life Galton was not his own best advocate for his theories. He had many long-lasting bouts of illness, and notwithstanding his and his wifes good intellectual pedigrees, they produced no children of their own to carry on his name and heritage. After his death in 1911, his will provided for the funding of a Chair of Eugenics and the Galton Eugenics Laboratory at the University of London.
The concept of improving the physical and mental characteristics of the human race may seem admirable at first glance. However, historically the method of achieving it has involved not just increasing the birthrate of the fit by selected parenthood (positive eugenics), but also reducing the birthrate of those people thought to impair such improvement, the unfit (negative eugenics).11
For example, by 1913, one-third (and from the 1920s on, more than half)12 of the US States had laws allowing for the compulsory sterilization of those held in custody who were deemed to be unfit. This resulted in the forced sterilization of some 70,000 victims, including criminals, the mentally retarded, drug addicts, paupers, the blind, the deaf, and people with epilepsy, TB or syphilis. Over 8,000 procedures were done at the one city of Lynchburg, Virginia,13 and isolated instances continued into the 1970s.14,15
About 60,000 Swedish citizen
s were similarly treated between 1935 and 1976, and there were similar practices in Norway and Canada.16
In Germany in 1933, Hitlers government ordered the compulsory sterilization of all German citizens with undesirable handicaps, not just those held in custody or in institutions. This was to prevent contamination of Hitlers superior German race through intermarriage.
Image Wikipedia.org
Eugenics congress logo. Click here for larger view
Then from 1938 to 1945, this surgical treatment of such useless eaters was superseded by a more comprehensive solutionthe eager genocide, by Hitlers Nazis, of over 11 million people considered to be subhuman or unworthy of life, as is authenticated and documented by the Nuremberg Trials records. Those killed included Jews, evangelical Christians,17 blacks, gypsies, communists, homosexuals, amputees and mental patients.
This was nothing other than rampant Darwinismthe elimination of millions of human beings branded unfit/inferior by, and for the benefit of, those who regarded themselves as being fit/superior.
The core idea of Darwinism is selection.18 The Nazis believed that they must direct the process of selection to advance the German race.19 Galtons nave vision of a eugenics utopia had mutated into the Nazi nightmare of murderous ethnic cleansing.
Sadly, ideas of racial superiority and eugenics did not die with Hitlers regime. David Duke, Americas infamous anti-black and anti-Jew racist, developed his views from reading the eugenicist writings of Galton, H.G. Wells, Sir Arthur Keith and others, as well as the early writings of modern sociobiologists such as Harvards E.O. Wilson.20
Following World War II, eugenics became a dirty word. Eugenicists now called themselves population scientists, human geneticists, family politicians, etc. Journals were renamed. Annals of Eugenics became Annals of Human Genetics, and Eugenics Quarterly became the Journal of Social Biology.21 However today, some 60 years after the Holocaust, the murderous concept that Galtons eugenics spawned is once again alive and flourishing, and wearing a lab-coat of medical respectability.
Doctors now routinely destroy humans, who were created in Gods image (Genesis 1:26), by abortion, infanticide and euthanasia, as well as in fetal/embryonic stem-cell research.
According to the UKs Daily Mail, women are increasingly eliminating their unborn children because of non life-threatening deformities such as deformed feet or cleft lips and palates, and more Downs Syndrome babies are now killed than are allowed to be born.22 Dr Jacqueline Laing of Londons Metropolitan University commented, These figures are symptomatic of a eugenic trend of the consumerist society hell-bent on obliterating deformity. This is straightforward eugenics, said UKs Life Trustee, Nuala Scarisbrick. The message is being sent out to disabled people that they should not have been born. It is appalling and abhorrent.22
Globally, there are an estimated 50 million abortions each year. Thats one abortion for every three live births, so any child in the womb, on average, worldwide, has a one in four chance of being deliberately killed.23
China is famous for its coercive one-child-per-family policy. In practice, most families want a boy, so if a girl is born, she can be at risk. Sometimes the same grisly principle is followed, but before birth. In India, its common to find out the sex of the baby, and a vast majority of abortions are of girl babies. It makes the feminist support of abortion distressingly ironic.
And disabled babies are at risk as well. Ethicist Peter Singer has advocated legalization of infanticide to a certain age. He writes: [K]illing a disabled infant is not morally equivalent to killing a person. Very often it is not wrong at all.24
In May 2001, Holland became the first country to legalize euthanasia, with the law coming into effect from January 2002. Euthanasia was tolerated in Belgium until May 2002, when it was legalized. It is tolerated in Switzerland, Norway and Columbia.23
Photo Bryan College
Clarence Darrow (left) and William Jennings Bryan
The textbook from which Scopes taught evolution, A Civic Biology by George Hunter,2 and its companion lab book3 were blatantly eugenic and offensively racist. Hunter divided humanity into five races and ranked them according to how high each had reached on the evolutionary scale, from the Ethiopian or negro type to the highest type of all, the Caucasians, represented by the civilized white inhabitants of Europe and America.4A Civic Biology asserted that crime and immorality are inherited and run in families, and said that these families have become parasitic on society. If such people were lower animals, we would probably kill them off to prevent them from spreading. Humanity will not allow this, but we do have the remedy of separating the sexes in asylums or other places and in various ways preventing intermarriage and the possibilities of perpetuating such a low and degenerate race.4
This is the book that Darwinists of the day insisted that Scopes had a right to teach!
All this is documented by Dr David Menton in the DVD Inherently Wind: a Hollywood History of the Scopes Trial (right).
Perhaps the most frequently asked question concerning the eugenics-inspired genocide of the Holocaust is: How could it have happened? In the 1961 MGM film Judgment at Nuremberg, about the trial of four Nazi war criminals, judges who had enforced Nazi decrees,1 one of the defendants (Judge Ernst Janning, played by Burt Lancaster) cries out to Chief Judge Dan Haywood (played by Spencer Tracy): Those peoplethose millions of peopleI never knew it would come to that. You must believe it! Haywoods response was eloquent: It came to that the first time you sentenced a man to death you knew to be innocent.
Likewise today, eugenic killing of innocent preborn babies because they are thought to be less than perfect began the first time a doctor consented to kill a handicapped child in the womb. The rest is history.
The photograph (above right) comes from the first Nuremberg Trial (19456), the most famous and significant of them because it tried the main German leaders. Front row (left-to-right): Hermann Gring, Rudolf Hess, Joachim von Ribbentrop, Wilhelm Keitel; Back row: Karl Dnitz, Erich Raeder, Baldur von Schirach, Fritz Sauckel. (Courtesy Wikipedia)
Not all evolutionists are murderers, of course, and Francis Galton may never have conceived that his theories would lead to the killing of so many millions of people, let alone the onslaught on defenceless unborn babies. However, such action is totally consistent with evolutionary teaching, namely the survival of the fittest by the elimination of the weakest. Deeds are the outcome of beliefs. As Jesus said: A bad tree bears bad fruit; it cannot bear good fruit (Matthew 7:1718).
Contrary to the deadly philosophy of eugenics, every human person has eternal value in Gods sight and has been created in the image of God (Genesis 1:2627). God also explicitly forbade murder (Exodus 20:13), or intentional killing of innocent humans. Indeed, God so loved humanity that He sent His Son, the Lord Jesus Christ, to die on the Cross to save us from sin (John 3:1617)
, and to transform us into the image of His Son when we believe on Him (Romans 8:29; 2 Corinthians 3:18). In Jesus, the Second Person of the Trinity took on human nature (Hebrews 2:14), becoming the Last Adam (1 Corinthians 15:45), thus becoming the (kinsman-) Redeemer (Isaiah 59:20) of the race of the first man, Adam.
(Also available in German, Polish and Russian)
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Eugenics ... death of the defenceless - creation.com
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The Missing Human Manual
Posted: March 2, 2016 at 3:44 pm
It is becoming more and more clear that our gut flora is the central issue for health. (More here on that)
It is best to start with the the healthiest gut flora possible. This means that it is best that we are born vaginally. We are a blank slate in the womb. Being born vaginally gives us our mothers flora.
Evidence is now coming out about how important this is. Leaving mothers with a more informed choice. If you can have a vaginal birth, you are giving your child the best start possible.
Here is the summary:
The researchers found that infants born by cesarean delivery were lacking a specific group of bacteria found in infants delivered vaginally, even if they were breastfed. Infants strictly formula-fed, compared with babies that were exclusively or partially breastfed, also had significant differences in their gut bacteria.
We want parents (and physicians) to realize that their decisions regarding c-section and breastfeeding can impact their infants gut microbiome, and this can have potentially lifelong effects on the childs health, says postdoctoral student and first author Meghan Azad, University of Alberta.
The potential long-term consequences of decisions regarding mode of delivery and infant diet are not to be underestimated, write the authors. Infants born by cesarean delivery are at increased risk of asthma, obesity and type 1 diabetes, whereas breastfeeding is variably protective against these and other disorders.
Beginning before birth, CHILD collects a range of information on environmental exposures such as pets, air pollution, household cleaning products, maternal and infant diet and more, and child health outcomes (including biological samples and clinical assessments). The researchers will use this information to study the development of the gut microbiome and its relationship to conditions such as wheeze and allergies in future studies.
Children born by cesarean delivery or fed with formula may be at increased risk of a variety of conditions later in life; both processes alter the gut microbiota in healthy infants, which could be the mechanism for the increased risk, writes Dr. Rob Knight, a Howard Hughes Medical Institute Early Career Scientist and an Associate Professor with the BioFrontiers Institute and Departments of Chemistry and Biochemistry and Computer Science, University of Colorado, Boulder, Colorado, United States, in a related commentary.
These issues are of direct relevance to pregnant women and health practitioners and should be considered when choices such as elective cesarean delivery and other interventions are discussed, state the commentary authors.
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The Missing Human Manual
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Mount Holly, New Jersey – Wikipedia, the free encyclopedia
Posted: at 3:44 pm
Mount Holly, New Jersey Township Township of Mount Holly Mount Holly Township highlighted in Burlington County. Inset map: Burlington County highlighted in the State of New Jersey. Census Bureau map of Mount Holly Township, New Jersey Coordinates: 395943N 744711W / 39.995351N 74.786452W / 39.995351; -74.786452Coordinates: 395943N 744711W / 39.995351N 74.786452W / 39.995351; -74.786452[1][2] Country United States State New Jersey County Burlington Formed November 6, 1688 as Northampton Incorporated February 21, 1798 Renamed November 6, 1931 as Mount Holly Named for Hill covered with holly trees Government[7] Type Faulkner Act (Council-Manager) Body Township Council Mayor Jason Jones (term ends December 31, 2016)[3][4] Township Manager Joshua Brown (Acting)[5] Clerk Nikima S. Muller [6] Area[1] Total 2.852sqmi (7.389km2) Land 2.806sqmi (7.269km2) Water 0.046sqmi (0.120km2) 1.63% Area rank 348th of 566 in state 31st of 40 in county[1] Elevation[8] 36ft (11m) Population (2010 Census)[9][10][11] Total 9,536 Estimate(2014)[12] 9,490 Rank 251st of 566 in state 16th of 40 in county[13] Density 3,397.9/sqmi (1,311.9/km2) Densityrank 191st of 566 in state 9th of 40 in county[13] Time zone Eastern (EST) (UTC-5) Summer (DST) Eastern (EDT) (UTC-4) ZIP code 08060[14][15] Area code(s) 609[16] FIPS code 3400548900[1][17][18] GNIS feature ID 0882104[1][19] Website twp.mountholly.nj.us
Mount Holly is a township in Burlington County, New Jersey, United States. It is the county seat of Burlington County[20][21] as well as an eastern suburb of Philadelphia. As of the 2010 United States Census, the township's population was 9,536,[9][10][11] reflecting a decline of 1,192 (-11.1%) from the 10,728 counted in the 2000 Census, which had in turn increased by 89 (+0.8%) from the 10,639 counted in the 1990 Census.[22] Mount Holly also gives its name to the National Weather Service's Weather Forecast Office for the Philadelphia metropolitan area, though the office is actually located in adjacent Westampton.[23][24]
What is now Mount Holly was originally formed as Northampton on November 6, 1688. Northampton was incorporated as one of New Jersey's first 104 townships by an act of the New Jersey Legislature on February 21, 1798. Portions of the township were taken to form Little Egg Harbor Township (February 13, 1740, now part of Ocean County), Washington Township (November 19, 1802), Pemberton borough (December 15, 1826), Coaxen Township (March 10, 1845, now known as Southampton Township), Pemberton Township (March 10, 1846), Westampton Township (March 6, 1850) and Lumberton Township (March 14, 1860). The township was renamed Mount Holly as of November 6, 1931, based on the results of a referendum held three days earlier.[25] The township was named for hills covered with holly trees.[26][27]
The first European settlement in what is now Mount Holly began in 1677, when Walter Reeves acquired land from the Lenape (Delaware) Native Americans living in the area. He constructed a dam on Rancocas Creek to channel water through a raceway to power a grist mill and saw mill.[28] Edward Gaskill and his sons hand dug the mill race on their property between 1720 and 1723.[29] After the mills were established, more settlers were attracted to the area and built houses and commercial buildings on High, Church, White, Mill, and Pine streets, including the Shinn Curtis Log House (1712). By 1800, over 250 dwellings had been built.[30]
Today no mills remain on the raceway, which still flows in its original course from the Rancocas just above the dam. The raceway proved a way for herring to make their way above the dam and was the scene of an annual fish run in the spring which provided fresh herring for slating and eating. The former mill land has been preserved as the Mill Dam Park. It marks the importance of mills to the early settlements.
On December 17, 1776, Colonel Samuel Griffin of the Continental Army crossed the Delaware River with 600 men mostly untrained men and boys, and with little equipment and marched to Mount Holly, where he set up a few "3-pounder" artillery pieces on Iron Works Hill. Hessian commanders von Block and Carl von Donop, were told that there were 3,000 American troops at Mount Holly.
By December 23, 1776, 2,000 Hessians were moved from Bordentown and positioned at The Mount in Mount Holly, where they engaged in a three-day-long artillery exchange, known as the Battle of Iron Works Hill or Battle of Mount Holly, with the Americans on Iron Works Hill. The Americans slipped away that night.[31]
After George Washington crossed the Delaware River on December 25, 1776, the fact that thousands of Hessian troops had been drawn to Mount Holly aided in the Continental Army's success in the Battle of Trenton the next day, a surprising American victory that helped turn the Army's fading morale after the disastrous defeat at the Battle of Fort Washington just weeks before and the ignominious retreat through New Jersey.[32]
The 1793 state legislature approved the relocation of the Burlington County seat from Burlington City to Mount Holly, which was approved by voters in a 1796 referendum.[33][34][pageneeded] Several important municipal buildings were constructed, including the courthouse in 1796 and the county prison built circa 1819. The Burlington County Prison was designed by Robert Mills, a nationally known architect who designed the Washington Monument. The town has numerous 18th and 19th-century buildings, most of which are included in the Mount Holly Historic District; it is listed in the New Jersey and National Register of Historic Places.[35] Commercial buildings were constructed primarily along High Street.
In 1849, the Burlington and Mount Holly Railroad was established, connecting communities along the Delaware River to Philadelphia, the major city of the area. The railroad supported industrialization along its route. The Camden and Mount Holly Railroad constructed a station 20 years later near the intersection of Washington and King streets.
A trolley station was built in 1904 for the passengers making connections to Burlington City and Moorestown. New municipal buildings were constructed during the 20th century, including the Town Hall on Washington Street (1930) and the U.S. Post Office (1935) located across the street (1935), both federally funded and constructed as Works Progress Administration projects under President Franklin D. Roosevelt during the Great Depression.
In the late 1950s, Mount Holly began to have economic difficulties due to industrial restructuring and the loss of working-class jobs. In the post-World War II period, numerous blue collar, family wage jobs disappeared as the community's traditional employers, the mills and dye factories, were shut down. At first these job losses were offset in part by gains at the nearby military bases, Fort Dix and McGuire Air Force Base, especially during the Vietnam War. In 1970, the residential vacancy rate in Mount Holly was 4.3%.
By 1980, however, the vacancy rate had climbed to 8.7% as a result of the nearby military installations' downsizing after the end of the Vietnam War. During this same period, 19701980, shopping malls proliferated in the suburban Philadelphia area, and retail business in Mount Holly suffered.[36] Mount Holly received Urban Enterprise Zone (UEZ) status in 1995; it has provided tax incentives and other assistance programs to local businesses, including lowering the sales tax rate to 3, half of the prevailing rate charges statewide.[37] This has helped to revive the local small business base.[37]
Mount Holly had a total area of 2.852 square miles (7.389km2), including 2.806 square miles (7.269km2) of land and 0.046 square miles (0.120km2) of water (1.63%).[1][2]
The township borders Eastampton Township, Hainesport Township, Lumberton Township, and Westampton Township.[38]
Clermont is an unincorporated community located within Mount Holly Township.[citation needed]
At the 2010 United States Census, there were 9,536 people, 3,456 households, and 2,264 families residing in the township. The population density was 3,397.9 per square mile (1,311.9/km2). There were 3,861 housing units at an average density of 1,375.8 per square mile (531.2/km2). The racial makeup of the township was 65.57% (6,253) White, 23.10% (2,203) Black or African American, 0.37% (35) Native American, 1.47% (140) Asian, 0.07% (7) Pacific Islander, 4.29% (409) from other races, and 5.13% (489) from two or more races. Hispanics or Latinos of any race were 12.69% (1,210) of the population.[9]
There were 3,456 households, of which 28.7% had children under the age of 18 living with them, 42.6% were married couples living together, 16.9% had a female householder with no husband present, and 34.5% were non-families. 27.4% of all households were made up of individuals, and 8.6% had someone living alone who was 65 years of age or older. The average household size was 2.61 and the average family size was 3.19.[9]
In the township, 23.5% of the population were under the age of 18, 9.6% from 18 to 24, 28.7% from 25 to 44, 27.1% from 45 to 64, and 11.1% who were 65 years of age or older. The median age was 36.3 years. For every 100 females there were 102.8 males. For every 100 females age 18 and over, there were 100.1 males.[9]
The Census Bureau's 2006-2010 American Community Survey showed that (in 2010 inflation-adjusted dollars) median household income was $53,841 (with a margin of error of +/- $4,427) and the median family income was $68,500 (+/- $4,684). Males had a median income of $51,945 (+/- $5,141) versus $37,079 (+/- $5,759) for females. The per capita income for the borough was $24,551 (+/- $1,785). About 7.1% of families and 12.2% of the population were below the poverty line, including 21.4% of those under age 18 and 8.8% of those age 65 or over.[52]
As of the 2000 United States Census[17] there were 10,728 people, 3,903 households, and 2,583 families residing in the township. The population density was 3,750.8 people per square mile (1,448.3/km). There were 4,248 housing units at an average density of 1,485.2 per square mile (573.5/km). The racial makeup of the township was 68.68% White, 21.57% African American, 0.42% Native American, 1.37% Asian, 0.07% Pacific Islander, 4.77% from other races, and 3.12% from two or more races. Hispanic or Latino of any race were 8.78% of the population.[50][51]
There were 3,903 households out of which 32.0% had children under the age of 18 living with them, 44.0% were married couples living together, 17.3% had a female householder with no husband present, and 33.8% were non-families. 27.2% of all households were made up of individuals and 10.0% had someone living alone who was 65 years of age or older. The average household size was 2.64 and the average family size was 3.20.[50][51]
In the township the age distribution of the population shows 26.3% under the age of 18, 9.4% from 18 to 24, 32.2% from 25 to 44, 19.6% from 45 to 64, and 12.4% who were 65 years of age or older. The median age was 35 years. For every 100 females there were 99.7 males. For every 100 females age 18 and over, there were 96.6 males.[50][51]
The median income for a household in the township was $43,284, and the median income for a family was $52,000. Males had a median income of $38,186 versus $27,425 for females. The per capita income for the township was $19,672. About 6.8% of families and 9.9% of the population were below the poverty line, including 11.4% of those under age 18 and 10.4% of those age 65 or over.[50][51]
Mount Holly Township operates within the Faulkner Act (formally known as the Optional Municipal Charter Law) under the Council-Manager (plan 12) form of municipal government, enacted by council-initiated action as of July 1, 1990.[53] Members of the township council are elected at-large in a partisan vote to serve four-year terms of office on a staggered basis, with either two or three seats up for election in even-numbered years as part of the November general election.[7][54] At a reorganization meeting after each election, the council selects a mayor and a deputy mayor from among its members. In November 2011, voters passed a referendum shifting from non-partisan municipal elections in May to partisan elections in November.[55]
As of 2015[update], members of the Mount Holly Township Council are Mayor Jason Jones (term on council ends December 31, 2016; term as Mayor ends 2016), Deputy mayor Richard DiFolco (term on council ends 2016; term as Deputy Mayor ends 2016), Lew Brown (2016), Betty Sykes (R, 2018) and Jules Thiessen (D, 2018).[3][56][57][58][59]
On May 11, 2010, voters of the Township elected Richard Dow, III and Dywnne Belton to Township Council, replacing incumbents Jules Thiessen and Brooke Tidswell, III, who served on the Council for 16 and 12 years, respectively. Dow received 557 votes, Belton 475, Christopher Sorhaindo, Dow's running mate, 470, Theissen, 377, and Tidswell, 353 votes.[60]
In July 2011, Township Council member Kimberly Kersey resigned.[61] In the November 2011 general election, Richard DiFolco was selected to fill Kersey's vacancy.[62]
In the November 2011 general election, voters approved a public question moving the municipal election from May to November in subsequent elections.[63]
On November 6, 2012, voters of the Township elected Lew Brown, Rich DiFolco and Jason Jones to 4-year terms on Town Council by a large margin, their terms will begin January 1, 2013.[64]
In January 2014, former mayor Richard Dow submitted his resignation as council member with one year remaining on his term of office.[65]
On March 31, 2014, five people filed petitions to appear on the primary ballot for two four-year terms for Township Council. Former mayor and current Mount Holly Municipal Utilities Authority Commissioner Jules Thiessen, BOE member Tim Young, and current Mount Holly Board of Education member and Planning Board Chairman Brian Grant filed to run for the democratic nominations. Wife of Mayor Rich DiFolco, Janet DiFolco, and Patricia Cauley filed for the republican nomination.[66]
In the November 2014 general election, Republican Elizabeth Sykes and Democrat Jules Thiessen were elected to four-year terms on the Township Council. Thiessen's running mate Brian Grant withdrew from the election in September as did both Republican candidates. Sykes replaced one of the republican candidates and no replacement was named for Grant making it an unopposed election. At the council's January 2015 reorganization, Jules Thiessen and Betty Sykes were sworn into office; Richard DiFolco was named Mayor and Jason Jones Deputy Mayor, both holding the same positions the previous year.[67]
Mount Holly Township is located in the 3rd Congressional District[68] and is part of New Jersey's 8th state legislative district.[10][69][70] Prior to the 2011 reapportionment following the 2010 Census, Mount Holly Township had been in the 7th state legislative district.[71]
New Jersey's 3rd Congressional District is represented by Tom MacArthur (R, Toms River).[72] New Jersey is represented in the United States Senate by Cory Booker (D, Newark, term ends 2021)[73] and Bob Menendez (D, Paramus, 2019).[74][75]
For the 20162017 session (Senate, General Assembly), the 8th Legislative District of the New Jersey Legislature is represented in the State Senate by Dawn Marie Addiego (R, Evesham Township) and in the General Assembly by Maria Rodriguez-Gregg (R, Evesham Township) and Joe Howarth (R, Evesham Township).[76] The Governor of New Jersey is Chris Christie (R, Mendham Township).[77] The Lieutenant Governor of New Jersey is Kim Guadagno (R, Monmouth Beach).[78]
Burlington County is governed by a Board of chosen freeholders, whose five members are elected at-large in partisan elections to three-year terms of office on a staggered basis, with either one or two seats coming up for election each year.[79] The board chooses a director and deputy director from among its members at an annual reorganization meeting held in January.[79] As of 2015[update], Burlington County's Freeholders are Director Mary Ann O'Brien (R, Medford Township, 2017; Director of Administration and Human Services),[80] Deputy Director Bruce Garganio (R, Florence Township, 2017; Director of Public Works and Health),[81]Aimee Belgard (D, Edgewater Park Township, 2015; Director of Hospital, Medical Services and Education)[82] Joseph Donnelly (R, Cinnaminson Township, 2016; Director of Public Safety, Natural Resources, and Education)[83] and Joanne Schwartz (D, Southampton Township, 2015; Director of Health and Corrections).[84][79] Constitutional officers are County Clerk Tim Tyler,[85] Sheriff Jean E. Stanfield[86] and Surrogate George T. Kotch.[87]
As of March 23, 2011, there were a total of 5,251 registered voters in Mount Holly Township, of which 1,718 (32.7% vs. 33.3% countywide) were registered as Democrats, 1,034 (19.7% vs. 23.9%) were registered as Republicans and 2,496 (47.5% vs. 42.8%) were registered as Unaffiliated. There were 3 voters registered to other parties.[88] Among the township's 2010 Census population, 55.1% (vs. 61.7% in Burlington County) were registered to vote, including 72.0% of those ages 18 and over (vs. 80.3% countywide).[88][89]
In the 2012 presidential election, Democrat Barack Obama received 2,636 votes here (68.1% vs. 58.1% countywide), ahead of Republican Mitt Romney with 1,127 votes (29.1% vs. 40.2%) and other candidates with 53 votes (1.4% vs. 1.0%), among the 3,870 ballots cast by the township's 5,578 registered voters, for a turnout of 69.4% (vs. 74.5% in Burlington County).[90][91] In the 2008 presidential election, Democrat Barack Obama received 2,771 votes here (67.2% vs. 58.4% countywide), ahead of Republican John McCain with 1,272 votes (30.8% vs. 39.9%) and other candidates with 58 votes (1.4% vs. 1.0%), among the 4,125 ballots cast by the township's 5,473 registered voters, for a turnout of 75.4% (vs. 80.0% in Burlington County).[92] In the 2004 presidential election, Democrat John Kerry received 2,223 votes here (57.2% vs. 52.9% countywide), ahead of Republican George W. Bush with 1,612 votes (41.5% vs. 46.0%) and other candidates with 37 votes (1.0% vs. 0.8%), among the 3,887 ballots cast by the township's 5,301 registered voters, for a turnout of 73.3% (vs. 78.8% in the whole county).[93]
In the 2013 gubernatorial election, Republican Chris Christie received 1,251 votes here (56.9% vs. 61.4% countywide), ahead of Democrat Barbara Buono with 891 votes (40.5% vs. 35.8%) and other candidates with 21 votes (1.0% vs. 1.2%), among the 2,200 ballots cast by the township's 5,429 registered voters, yielding a 40.5% turnout (vs. 44.5% in the county).[94][95] In the 2009 gubernatorial election, Democrat Jon Corzine received 1,126 ballots cast (49.6% vs. 44.5% countywide), ahead of Republican Chris Christie with 977 votes (43.1% vs. 47.7%), Independent Chris Daggett with 118 votes (5.2% vs. 4.8%) and other candidates with 38 votes (1.7% vs. 1.2%), among the 2,269 ballots cast by the township's 5,524 registered voters, yielding a 41.1% turnout (vs. 44.9% in the county).[96]
For pre-Kindergarten through eighth grade, students attend the Mount Holly Township Public Schools. As of the 2011-12 school year, the district's three schools had an enrollment of 905 students and 87.8 classroom teachers (on an FTE basis), for a studentteacher ratio of 10.31:1.[97] Schools in the district (with 2011-12 enrollment data from the National Center for Education Statistics[98]) are John Brainerd School[99] (356 students in grades PreK-2), Gertrude C. Folwell School[100] (247 students in grades 3-5) and F. W. Holbein Middle School[101] (302 students in grades 6-8).[102][103]
For ninth through twelfth grades, public school students attend the Rancocas Valley Regional High School, a comprehensive regional public high school based in Mount Holly that serves students from five communities encompassing an area of 40 square miles (100km2) that also includes the communities of Eastampton Township, Hainesport Township, Lumberton Township and Westampton Township.[104][105][106]
Students from Mount Holly Township, and from all of Burlington County, are eligible to attend the Burlington County Institute of Technology, a countywide public school district that serves the vocational and technical education needs of students at the high school and post-secondary level at its campuses in Medford and Westampton Township.[107]
As of May 2010[update], the township had a total of 38.43 miles (61.85km) of roadways, of which 29.11 miles (46.85km) were maintained by the municipality, 8.45 miles (13.60km) by Burlington County and 0.87 miles (1.40km) by the New Jersey Department of Transportation.[108]
Mount Holly is accessible at exit 5 of the New Jersey Turnpike via County Route 541.[109]
New Jersey Transit provides bus service to Philadelphia on routes 317 (from Asbury Park) and 409/417/418 (from Trenton), with local service available on the 413 route between Camden and Burlington.[110][111]
People who were born in, residents of, or otherwise closely associated with Mount Holly include:
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Mount Holly, New Jersey - Wikipedia, the free encyclopedia
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United Nations Envisions Transhumanist Future Where Man is …
Posted: at 3:43 pm
Aaron Dykes Infowars.com June 10, 2012
The Global Future 2045 International Congress, led by iconic futurist Ray Kurzweil and held in Moscow a few months back, lays out a stark vision of the future for neo-humanity where AI, cybernetics, nanotech and other emerging technologies replace mankind an openly transhumanist vision now being steered by the elite, but which emerged out of the Darwinian-circles directed by the likes of T.H. Huxley and his grandchildren Julian, who coined the term Transhumanism, and Aldous Huxley, author of Brave New World. Resistance to this rapid shift in society, the 2045 conference argues, is nothing short of a return to the middle ages.
As the video points out, the group admittedly met to draft resolution that will be submitted to the United Nations demanding the implementation of committees to discuss life extension Avatar projects as a necessary tool in the preservation of humankind.
2045: A New Era for Humanity
Russia 2045 dubs itself a strategic social movement, with aims to evolve humanity and extend life towards the everlasting. The project outlines a forecast for development in the following increments:
Now: the emergence of new Transhumanist movements & parties amid the ongoing socio-economic crisis between 2012-2013; new centers for cybernetic technologies to radically extend life, where the race for immortality starts by 2014, the creation of the avatar (robotic human copy) between 2015-2020, as well as robots to replace human manufacturing & labor, servant tasks; thought controlled robots to displace travel needs; flying cars, thought-driven communications implanted in bodies or sprayed on skin. By 2025, the group foresees the creation of an autonomous system providing life support for the brain that is capable of interacting with the environment; brains transplanted into avatar bodies greatly expanding life and allowing complete sensory experiences. Between 2030-2035, the emergence of Re-Brain, a reverse-engineering of the human brain already being mapped out, wherein science comes close to understanding the principles of consciousness. By 2035, the first successful transplantation of personality to other data receptacles and the epoch of cybernetic immortality begins. 2040-2050 brings the arrival of bodies made of nano-robots that can take any shape, as well as hologram bodies. 2045-2050 will bring forth drastic changes to the social structure and sci-tech development. It is in this age that the United Nations original promise of the end to war & violence is again predicted, where instead spiritual self-improvement takes precedent. A New Era of Neo-Humanity Dawns, according to the video.
This is textbook Transhumanism, rooted in many ancient orders and the philosophy of eugenics.
At its heart, Transhumanism represents an esoteric quest for godhood among certain circles of the elite connected to masonry, occultism and science/technology wherein supposedly evolving, superior beings ethically replace lesser humans. This philosophy is portrayed in this summers blockbuster Prometheus, a sort of prequel to the Alien series, and directed by Sir Ridley Scott, who founded the film franchise. See Alexs highly accurate breakdown of the themes behind the movie below, which help illustrate the dangers of emerging technology in the hands of the elite who hold this vision:
Secrets of Prometheus Film Leaked
Fittingly, two of the attendees at the 2012 anglophile Bilderberg meeting were Russians dealing with science & technology (though neither were apparently involved directly in this 2045 conference) including the owner of a Nano technology company, while Bilderberg steering committee members like Silicon Valley exec Peter Thiel are funding private space ventures, artificial island civilizations, next-gen Internet ventures and more.
RUS Chubais, Anatoly B. CEO, OJSC RUSNANO RUS Ivanov, Igor S. Associate member, Russian Academy of Science; President, Russian International Affairs Council
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United Nations Envisions Transhumanist Future Where Man is ...
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The United States and NATO
Posted: at 5:45 am
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The United States and NATO
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Kids.Net.Au – Encyclopedia > NATO
Posted: at 5:45 am
The North Atlantic Treaty Organization (NATO) is an international organization for defence collaboration established in 1949, in support of the North Atlantic Treaty signed in Washington, D.C. on April 4, 1949.
The core provision of the treaty is Article V, which states:
This provision was intended so that if the Soviet Union launched an attack against the European allies of the United States, it would be treated as if it was an attack on the United States itself. However the feared Soviet invasion of Europe never came. Instead, the provision was used for the first time in the treaty's history on September 12, 2001 in response to the September 11, 2001 Terrorist Attack.
Member States From the foundation in 1949 or with the year of accession.
Greece and Turkey joined the organization in February 1952. Germany joined as West Germany in 1955 and German unification in 1990 extended the membership to the areas of former East Germany. Spain was admitted on May 30, 1982 and the former Warsaw Pact Countries of Poland, Hungary and the Czech Republic made history by becoming members on March 12, 1999.
France is still a member of NATO but retired from the military command in 1966. Iceland, the sole member of NATO which does not have its own military force, joined on the condition that they would not be forced to participate in warfare.
History
On March 17, 1948 Benelux, France, and the United Kingdom signed the Treaty of Brussels[?] which is a precursor to the NATO Agreement.
The Soviet Union and its satellite states formed the Warsaw Pact in the 1950s in order to counterbalance NATO. Both organisations were opposing sides in the cold war. After the fall of the Iron Curtain in 1989, the Warsaw Pact disintegrated.
NATO saw its first military engagement in the Kosovo War, where it waged an 11-week bombing campaign against Serbian forces starting on March 24, 1999.
Three former communist countries, Hungary, the Czech Republic and Poland, joined NATO in 1999. At the Prague (Czech Republic) summit of November 21-22, 2002 seven countries have been invited to start talks in order to join the Alliance: Estonia, Latvia, Lithuania, Slovenia, Slovakia, Bulgaria and Romania. The invited countries are expected to join NATO in 2004. Albania and the Former Yugoslav Republic of Macedonia will probably be told they have not met the economic, political and military reform criteria and will have to wait. Croatia applied only in 2002 and has just started the process.
Charles de Gaulle's decision to remove France from NATO's military command in 1966 to pursue its own nuclear defence program precipitated the relocation of the NATO Headquarters from Paris, France to Brussels, Belgium by October 16, 1967. While the political headquarters is located in Brussels the military headquarters, the Supreme Headquarters Allied Powers Europe (SHAPE), are located just south of Brussles, in the town of Mons.
September 13, 2001, NATO invoked, for the first time in its history, an article in its charter that states that any attack on a member state is considered an attack against the entire alliance. This came in response to the September 11, 2001 Terrorist Attack/
On February 10, 2003 NATO faced a serious crisis because of France and Belgium breaking the procedure of silent approval concerning the timing of protective measures for Turkey in case of a possible war with Iraq. Germany did not use its right to break the procedure but said it supported the veto.
On April 16, 2003, NATO agreed to take command in August of the International Security Assistance Force (ISAF) in Afghanistan. The decision came at the request of Germany and the Netherlands, the two nations leading ISAF at the time of the agreement. It was approved unanimously by all 19 NATO ambassadors. This marked first time in NATO's history that it took charge of a mission outside the north Atlantic area. Canada had originally been slated to take over ISAF in August.
See also: Euro-Atlantic Partnership Council, OSCE, WEU, UN
All Wikipedia text is available under the terms of the GNU Free Documentation License
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Kids.Net.Au - Encyclopedia > NATO
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Liberty Resources
Posted: at 5:42 am
Liberty Resources, Inc. is a not-for-profit, Consumer-controlled organization that advocates and promotes independent living for all persons with disabilities. As a Center for Independent Living (CIL), Liberty Resources advocates with disabled people, individually and collectively to ensure our civil rights and equal access to all aspects of life in the community.
Liberty Resources must provide four core services: Advocacy, Information and Referral, Peer Support and Skills Training. Click to read more about the core services. In addition to those, a CIL should respond to the unique needs of its community. Liberty Resources is one of the first Centers for Independent Living in Pennsylvania, and has been consistently able to add services to address the needs of our community. Read more about the other services that Liberty Resources has added to its menu.
Liberty Resources Home Choices
Liberty Resources Home Choices provides a full range of in-home care services including, but not limited to, Personal Care, Homemaking/Light Housekeeping and Companionship. Home care services are non-medical. Click here to learn more.
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Liberty Resources
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