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I-5-1 Basic Principles and Components of PCR NSYSU CHUNG-LUNG CHO.

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Presentation on theme: "I-5-1 Basic Principles and Components of PCR NSYSU CHUNG-LUNG CHO."— Presentation transcript:

1 I-5-1 Basic Principles and Components of PCR NSYSU CHUNG-LUNG CHO

2 I-5- 2 Published papers with ‘ PCR ’ 1989 - 219 1990 – 4961998,10 - >73,000 1991 – 7111999,4 - >81,000 1992 – 9062000,10 – 121,305 1993 –10302001,2 – 125,563 1994 – 857 (>4000) 2002,3 – 149,572 1995 – 8232003,2 – 170,841 1996 – 7962004,2,23-195,193 1997 – 7322004,2,26-195,265 2006,3,22 - 255,788 2006/4/18 – 257,737 2007/3/9 – 283,607 2007/4/11 - 286,486

3 I-5- 3 1985 Enzymatic amplification of beta-globin genomic sequences and restriction site analysis for diagnosis of sickle cell anemia. Science. 1985 Dec 20;230(4732):1350-4. Saiki RK, Scharf S, Faloona F, Mullis KB, Horn GT, Erlich HA, Arnheim N. Cetus Corporation, Department of Human Genetics, Emeryville, CA 94608.

4 I-5- 4 PCR: Polymerase Chain Reaction A method of in vitro cloning Allows amplification of specific DNA molecules (fragments) in vitro through cycles of enzymatic DNA synthesis The most popular and widely used technique in all fields of biological studies probably. Why?

5 I-5- 5 1. simple 2. powerful  A. sensitive – sensitivity  B. specific – specificity  C. reliable – reliability; fidelity 3. fast

6 I-5- 6 DNA Replication Purpose: To duplicate DNA molecule Principle:  Separation of DNA double-stranded template  Primer formation  Extension of new DNA strands by a DNA polymerase and deoxyribonucleoside triphosphates (dNTPs)  Other proteins involved

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9 I-5- 9 Principle of PCR Purpose: Condition: Components:

10 I-5- 10 Purpose To amplify a lot of double-stranded DNA molecules (fragments) with same (identical) size and sequence by enzymatic method and cycling condition.

11 I-5- 11 Condition 1. Denaturation of ds DNA template 2. Annealing of primers 3. Extension of ds DNA molecules

12 I-5- 12 Denaturation Melt of ds DNA Tm: melting temperature Consequences of DNA Strands Separation Decrease in hydrophobic interactions between DNA bases Increase in UV absorbance

13 I-5- 13 Annealing Hybridize Primers anneal to denatured template DNA Tm of primers Annealing temperature

14 I-5- 14 Extension DNA polymerase synthesizes (polymerizes) new DNA molecule by adding deoxyribonucleoside complementary to the corresponding template base in a 5’ to 3’ direction.

15 I-5- 15 Cycling Cycle number Ramp time

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18 I-5- 18 Chemical Components Enzyme Buffers and MgCl 2  100 mM Tris-HCl, pH 8.3  500 mM KCl  15 mM MgCl 2  0.1% gelatin Deoxynucleoside triphosphates (dNTPs) Template DNA Primers

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22 I-5- 22 Instrumentation

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25 I-5- 25 Consumables

26 I-5- 26 Three Aspects of PCR Specificity Efficiency Fidelity

27 I-5- 27 The best way to understand PCR is to consider the reaction components and how they combine to produce the best results. Each physical and chemical components of PCR can be modified to produce a potential increase in yield, specificity, or sensitivity.

28 I-5- 28 Development/Invention of PCR Technique 1993 Nobel Prize in Chemistry

29 I-5- 29 Unusual Origin of PCR, Mullis KB, Scientific American 1990,56

30 I-5- 30

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