Show the calculations for the preparation of 0.01%, 0.001%, 0.0001%, 0.00001% standard DNA solutions via serial dilution from a 0.1% stock solution.   Prepare 10.0 mL of 0.10% standard DNA solution using acetate buffer pH 4.6 as solvent. Prepare four different concentrations of the 0.10% standard DNA solution from step 1 via serial dilution to obtain 0.01%, 0.001%, 0.0001%, 0.00001% standard DNA solutions. Obtain seven clean and dry test tubes. Place 1.50 mL solutions in each tube as follows:   Table 2.1. Set-up for the diphenylamine assay.   Test tube # Content 1 (blank) acetate buffer pH 4.6 2 0.10% standard DNA 3 0.01% standard DNA 4 0.001% standard DNA 5 0.0001% standard DNA 6 0.00001% standard DNA 7 DNA extract from Part I   Add 3.50 mL diphenylamine reagent to each tube, swirl each tube to thoroughly mix the contents and heat for 10 mins in a boiling water bath. Cool immediately under tap water. Read absorbances at 595 nm. Construct the standard curve and determine the concentration of the DNA in the tissue extract from the standard curve. If the concentration of the DNA extract does not fall within the range of the calibration curve, dilute the sample and re-read its absorbance.

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Author:Elaine N. Marieb, Katja N. Hoehn
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Chapter1: The Human Body: An Orientation
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Show the calculations for the preparation of 0.01%, 0.001%, 0.0001%, 0.00001% standard DNA solutions via serial dilution from a 0.1% stock solution.

 

  1. Prepare 10.0 mL of 0.10% standard DNA solution using acetate buffer pH 4.6 as solvent.
  2. Prepare four different concentrations of the 0.10% standard DNA solution from step 1 via serial dilution to obtain 0.01%, 0.001%, 0.0001%, 0.00001% standard DNA solutions.
  3. Obtain seven clean and dry test tubes. Place 1.50 mL solutions in each tube as follows:

 

Table 2.1. Set-up for the diphenylamine assay.  

Test tube #

Content

1 (blank)

acetate buffer pH 4.6

2

0.10% standard DNA

3

0.01% standard DNA

4

0.001% standard DNA

5

0.0001% standard DNA

6

0.00001% standard DNA

7

DNA extract from Part I

 

  1. Add 3.50 mL diphenylamine reagent to each tube, swirl each tube to thoroughly mix the contents and heat for 10 mins in a boiling water bath. Cool immediately under tap water.
  2. Read absorbances at 595 nm.
  3. Construct the standard curve and determine the concentration of the DNA in the tissue extract from the standard curve. If the concentration of the DNA extract does not fall within the range of the calibration curve, dilute the sample and re-read its absorbance.

 

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