Abstract

A method to detect and quantify polymerase chain reaction (PCR) product from a DNA target fragment associated with Acquired Immunodeficiency Syndrome (AIDS) was developed. The current method to detect PCR product is by Agarose Gel Electrophoresis and staining with ethidium bromide, but quantitation is by the operator's estimation. As a result of this project, the PCR product can be detected by High Pressure Liquid Chromatography (HPLC) and the amount of product can be determined by using an internal standard. By detection of the PCR product on the HPLC and subsequent quantitation, the efficiency of the PCR can be determined. Samples from different PCR experiments (all using the HIV-1 target fragment) were tested using the HPLC method to determine the product's concentration.

Library of Congress Subject Headings

Polymerase chain reaction--Diagnostic use; AIDS (Disease)--Research; Liquid chromatography--Diagnostic use; DNA probes--Diagnostic use

Publication Date

1-1990

Document Type

Thesis

Student Type

Graduate

Advisor

Name(s) Illegible

Comments

Physical copy available from RIT's Wallace Library at QP606.D46 L375 1990

Recommended Citation

LaTart, David Brewer, "Quantitative determination of polymerase chain reaction product for HIV-1" (1990). Thesis. Rochester Institute of Technology. Accessed from
https://repository.rit.edu/theses/8429

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Quantitative determination of polymerase chain reaction product for HIV-1

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Theses

Quantitative determination of polymerase chain reaction product for HIV-1

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Abstract

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