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Clinical Chemistry, Vol 42, 1582-1588, Copyright © 1996 by American Association for Clinical Chemistry
RC McGlennen
Department of Laboratory Medicine and Pathology, University of Minnesota Health System, Minneapolis 55455, USA. mcgle001@maroon.tc.umn.edu
Routine clinical molecular testing of diseases associated with unstable or dynamic trinucleotide repeat syndromes poses unique technical, medical, and ethical challenges to the laboratory. Although the pathophysiology of these disorders is to date still largely undefined, the uniformity of their genetics has led to the development of highly informative diagnostic tests. In general, amplification techniques, such as the polymerase chain reaction (PCR), are used to determine the size of alleles within the genes linked to these disorders. Technically, these assays require empirical optimization so that the PCR reactions are both robust and reproducible, and occasionally other methods must be used to confirm diagnoses. Beyond execution of the test, however, the molecular diagnostics laboratory needs also to be fundamentally involved in the process of interpreting these tests in the correct clinical context and in setting policy as to how these data are presented to patients.
The following articles in journals at HighWire Press have cited this article:
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  B. Melegh and J. Molnar Nonisotopic Method for Precise Detection of (CAG)n Repeats Clin. Chem., June 1, 1997; 43(6): 1096 - 1097. [Full Text] [PDF]
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