The amount of each component for a PCR reaction is critical. The final concentration of each primer should be 0.2 uM, and the final concentration of dNTPs is 0.2 mM. If the final concentrations of these components are significantly off, your PCR reactions will not work. The stock concentration of primers is usually 10 uM and the stock concentration of dNTPs is usually 10 mM. PCR buffer is supplied as 10X and should be 1X in the final reaction volume. The amount of Taq DNA polymerase necessary will depend on the manufacturer. For our purposes, Taq polymerase is supplied at a concentration of 20 Units/ ul. Each PCR reaction should include 5 units of Taq polymerase. 1) Calculate the necessary volume to set up a single PCR reaction given the following: Assume you will use 2 ul of template DNA (e.g. isolated from a patient). You have the following primer stocks GAPDH Forward Primer, 10 uM stock GAPDH Reverse Primer, 10 uM stock SARS-CoV-2 Forward Primer, 10 uM stock SARS-CoV-2 Reverse Primer, 10 uM stock 10X PCR Reaction Buffer dNTPs, 10 mM stock Taq polymerase, 20 Units/uL stock The final reaction volume should be 30 ul 2) Now, calculate what is needed to run samples for five patients plus a negative, no-template control sample. In your notebook, plan the pooled reaction that would be required to run these six PCR reactions. Remember that a pooled reaction should only include components common to all reactions and that you need to mix enough for one extra reaction to account for errors in pipetting.

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The amount of each component for a PCR reaction is critical. The final concentration of each primer should be 0.2 uM, and the final concentration of dNTPs is 0.2 mM. If the final concentrations of these components are significantly off, your PCR reactions will not work. The stock concentration of primers is usually 10 uM and the stock concentration of dNTPs is usually 10 mM. PCR buffer is supplied as 10X and should be 1X in the final reaction volume. The amount of Taq DNA polymerase necessary will depend on the manufacturer. For our purposes, Taq polymerase is supplied at a concentration of 20 Units/ ul. Each PCR reaction should include 5 units of Taq polymerase.

1) Calculate the necessary volume to set up a single PCR reaction given the following:


Assume you will use 2 ul of template DNA (e.g. isolated from a patient).

You have the following primer stocks

GAPDH Forward Primer, 10 uM stock

GAPDH Reverse Primer, 10 uM stock

SARS-CoV-2 Forward Primer, 10 uM stock

SARS-CoV-2 Reverse Primer, 10 uM stock

10X PCR Reaction Buffer dNTPs, 10 mM stock

Taq polymerase, 20 Units/uL stock

The final reaction volume should be 30 ul

2) Now, calculate what is needed to run samples for five patients plus a negative, no-template control sample. In your notebook, plan the pooled reaction that would be required to run these six PCR reactions. Remember that a pooled reaction should only include components common to all reactions and that you need to mix enough for one extra reaction to account for errors in pipetting.

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