Platinum™ GenoType Tsp DNA Polymerase
Platinum&trade; GenoType <i>Tsp</i> DNA Polymerase
Invitrogen™

Platinum™ GenoType Tsp DNA Polymerase

Platinum GenoType Tsp DNA Polymerase is designed and qualified specifically for amplification of dinucleotide repeat markers in PCR-based genotyping applications.
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11448024400 Reactions
11448032
11448-032으로도 사용됨
2000 Reactions
카탈로그 번호 11448024
제품 가격(KRW)
629,000
Exklusiv online
Ends: 31-Mar-2026
740,000
할인액 111,000 (15%)
Each
카트에 추가하기
반응 수:
400 Reactions
제품 가격(KRW)
629,000
Exklusiv online
Ends: 31-Mar-2026
740,000
할인액 111,000 (15%)
Each
카트에 추가하기
Platinum GenoType Tsp DNA Polymerase is designed and qualified specifically for amplification of dinucleotide repeat markers in PCR-based genotyping applications. The enzyme is pre-complexed with a thermolabile inhibitor containing monoclonal antibodies to Tsp DNA polymerase, providing an automatic hot-start method that improves PCR specificity and allows for room temperature reaction assembly.

Platinum GenoType Tsp DNA Polymerase features

  • Minimal non-templated nucleotide addition to PCR products
  • Lacks both 5' and 3' exonuclease activity
  • Amplifies fragments up to 500 bp
  • Room temperature reaction assembly

Application

Amplification of dinucleotide repeat loci in applications in which elimination of non-templated nucleotide addition is desirable.

Unit definition

One unit of Platinum GenoType Tsp DNA Polymerase has been functionally determined to be equivalent to one unit of Taq DNA Polymerase in amplification of dinucleotide repeats using standard Taq DNA polymerase reaction conditions. One Tsp DNA polymerase unit approximates 2.5 activity units. An activity unit incorporates 10 nmoles of deoxyribonucleotide into acid-precipitable material in 30 min. at 74°C under optimized reaction conditions.

For Research Use Only. Not for use in diagnostic procedures.
사양
Fidelity (Taq 대비)1X
핫 스타트Built-In Hot Start
반응 수400 Reactions
오버행Blunt
중합효소Tsp Genotyping Polymerase
수량250 units
반응 형식Separate Components
배송 조건Wet or Dry Ice
크기(최종 제품)500 bp or less
부피50 μL
용도(애플리케이션)Hot-start PCR
GC-Rich PCR PerformanceLow
반응 속도Standard
Unit SizeEach
구성 및 보관
• Platinum GenoType Tsp DNA Polymerase (50 μL at 5 Tsp U/μL)
• 10X PCR Buffer (1.25 mL)
• 50 mM MgCl2 (1 mL)

Store at -20°C. Guaranteed stable for 6 months when properly stored.

자주 묻는 질문(FAQ)

What is the difference between Platinum technology and AccuPrime technology?

With Platinum technology, anti-DNA polymerase antibodies bind to the enzyme until the denaturing step at 94 degrees C, when the antibodies degrade. The polymerase is now active and primer extension can occur. AccuPrime Taq combines Platinum Taq (Taq + Platinum antibodies) with proprietary thermostable AccuPrime accessory proteins. The 10X reaction buffer contains the accessory proteins which enhance specific primer-template hybridization during each cycle of PCR.

Is there anything to prevent AmpliTaq Gold DNA polymerase from extending from the 3’ end of a TaqMan probe in a 5’ nuclease assay?

Yes. There is a phosphate group on the 3' end of all TaqMan probes that prevents such extension.

How does AmpliTaq Gold DNA Polymerase differ from AmpliTaq DNA Polymerase?

AmpliTaq Gold DNA Polymerase is a modified form of AmpliTaq DNA Polymerase that contains a proprietary chemical (or so-called hot start molecule) bound to the enzyme's active site. In order to activate the AmpliTaq Gold DNA Polymerase fully, we recommend an initial activation step of 95 degrees C for 10 min when using GeneAmp 10X PCR Buffer I and/or GeneAmp 10X PCR Buffer II and Mg in one of our thermal cyclers. When using GeneAmp 10X PCR Gold Buffer, activation time can be reduced to 5 minutes. Once activation is complete, you can proceed with your standard PCR cycling program (denaturing, annealing, extension, etc).

Does AmpliTaq Gold DNA Polymerase contain exonuclease (proofreading) activity?

No, AmpliTaq Gold DNA polymerase does not contain proofreading activity, however fidelity in PCR amplifications utilizing this enzyme may be improved. High fidelity can be achieved by: 1. Decreasing the final concentration of each nucleotide to 40-50 uM. 2. Using the lowest MgCl2 concentration possible. 3. Using less enzyme. 4. Decreasing extension times. 5. Using the highest annealing temperature possible. 6. Using as few cycles as possible.

Does the fidelity of AmpliTaq DNA Polymerase change in the presence of base analogs?

The fidelity of this PCR enzyme is affected in two ways. First, AmpliTaq DNA Polymerase typically binds to and incorporates base analogs less efficiently than conventional dNTPs, which means that polymerase activity is lower in reactions that contain base analogs. Second, the analog may pair with more than one conventional complementary template base, so the analog may be incorporated at an increased level compared to conventional dNTPs. For the best fidelity, we recommend that base analogs are included at low concentrations in the reaction.

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