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Simplified Algorithms for Determining Cycle Shift between qPCR Fluorescence Curves
Author(s) -
Michael E. Jones,
George C. Mayne,
Tingting Wang,
David I. Watson,
Damian J. Hussey
Publication year - 2015
Publication title -
computational biology journal
Language(s) - English
Resource type - Journals
eISSN - 2314-4173
pISSN - 2314-4165
DOI - 10.1155/2015/601504
Subject(s) - dna , fluorescence , algorithm , computation , biological system , chemistry , biology , mathematics , physics , biochemistry , optics
This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.The polymerase chain reaction is a central component of current molecular biology. It is a cyclic process, in each early cycle of which the template DNA approximately doubles. An indicator which fluoresces when bound to DNA quantifies the DNA present at the end of each cycle, giving rise to a fluorescence curve which is characteristically sigmoid in shape. The fluorescence curve quantifies the amount of DNA initially present; the more the initial DNA, the earlier the rise in the fluorescence. Accordingly the amount of DNA initially present in two samples can be compared: the sample with the less DNA gives rise to a relatively delayed fluorescence curve and the ratio of the DNAs can be deduced from the separation of the curves. There is, however, a second determinant of this separation, the fold increase in DNA per cycle: ideally a twofold increase but frequently less. Current guidelines recommend that this be determined experimentally by carrying out PCR on a series of dilutions. If the value of the fold increase is known, then the algorithm for determining the separation can be reduced to a relatively simple computation, rather than employing a multidimensional nonlinear optimization such as the Marquardt-Levenberg as currently employed

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