can anyone please illustrate the whole protocol of sanger sequencing in simple way that involves purification of PCR reaction, bigdye PCR reaction, purification...or please recommend any site which can clear the concepts....why each step is being done and the purpose of different reagents....i am specially confused about the PCR reaction that includes bigdye that how this reaction do the amplification as no polymerase and other reagents are added?
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Originally posted by quratulain View Post.i am specially confused about the PCR reaction that includes bigdye that how this reaction do the amplification as no polymerase and other reagents are added?
Please note that reaction, although performed on a thermal cycler, is not a PCR reaction. The "chain reaction" of PCR occurs because the products of one cycle become templates in the next. PCR leads to an exponential increase in target DNA amounts. A normal sequencing reaction includes only a single oligonucleotide to prime polymerization. By cycling the reaction you can linearly increase the number of product molecules produced. But these product molecules are not templates for subsequent cycles.
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Phillip
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sequencing protocol
thanks alot... by saying "A normal sequencing reaction includes only a single oligonucleotide to prime polymerization", you mean , we use only one primer?Last edited by quratulain; 12-15-2014, 10:24 AM.
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Originally posted by quratulain View Postthen what is meant by forward and reverse primer? they are not two?
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Phillip
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after the sequencing reaction in thermal cycler, are the products double stranded and as due to addition of ddnTPs, the reaction stops, so one strand will have ddnTP at its 3 prime end while other strand does not have ddnTP at its 3 prime end but regular dnTP, i am right? and are these double stranded products denatured in the genetic analyzer before detection by laser?
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Originally posted by quratulain View Postafter the sequencing reaction in thermal cycler, are the products double stranded and as due to addition of ddnTPs, the reaction stops, so one strand will have ddnTP at its 3 prime end while other strand does not have ddnTP at its 3 prime end but regular dnTP, i am right? and are these double stranded products denatured in the genetic analyzer before detection by laser?
No, we no longer denature these double stranded products, mainly because of cycle-sequencing.
With cycle-sequencing each template strand produces many product strands. As many as 1 new product strand per thermal cycle. For this reason, the ratio of product to template strands is high. >10:1. So denaturation isn't necessary as there is already a large pool of single stranded products present in the final reaction.
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Phillip
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but i don't understand that as products would be double stranded upto the position the ddnTP is incorporated and then single stranded, does all products would be not like that? denaturation isn't necessary as there is already a large pool of single stranded products present in the final reaction, from where only single stranded comes, they are not double stranded upto the position the ddnTP is incorporated and then single stranded?
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Yes, but at the beginning of each cycle the product strands from the previous cycle are melted from the template strands.
Details:
The sample starts out as normal double stranded DNA. The first step of cycle sequencing heats the sample up and the strands denature. Now the sample is single-stranded. Then the next step cools the sample so that the sequencing primers anneal to a specific place on the single stranded template. The temp is again adjusted so that the polymerases become active and extend the primers until they incorporate a ddNTP. That is the end of the cycle. Maximum possible yield: one product strand (of variable length) per template.
The second cycle begins as the first did, with a denaturation step. This melts all the product strands from all the template strands. Primer can anneal, etc.
Each cycle, the pool of product strands increases. So, at the end, even if a product strand anneals to each template, there will be plenty of extra product still left without template available to anneal to.
The truth is, in ancient times, 10+ years ago, many of us denatured samples just before loading them on the sequencer. But it was found not to be necessary, so these days most people don't bother.
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Phillip
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Originally posted by quratulain View Postcan i sequence 44 samples at a time in 3130 ABI genetic analyzer and how long will it take for their capillary electrophoresis?
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Phillip
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