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Quantitation of in situ hybridization of ribosomal ribonucleic acids to human diploid cells
Authors:Babette D Coté  Olke C Uhlenbeck  Dale M Steffensen
Institution:(1) Department of Biochemistry, University of Illinois, 61801 Urbana, Illinois;(2) Department of Genetics and Development, University of Illinois, 61801 Urbana, Illinois;(3) Present address: Department of Physiological Chemistry, University of Wisconsin, 53706 Madison, Wisconsin, USA
Abstract:The hybridization of 5S and 28S ribosomal RNAs to human fibroblast and leukocyte cells was used as a model system to quantitate the technique of in situ hybridization for human diploid cell types. Quantitation consisted of counting (scoring) the number of grains formed over both interphase nuclei and metaphase chromosomes on slides after various hybridization procedures. The average number of grains/nucleus per slide was then used to determine hybridization percentages. As with nitrocellulose filter hybridizations the kinetics of in situ hybridizations can be fit with a single first-order rate constant. However, the in situ hybridization rate was approximately 10 times slower than the corresponding filter hybridization rate. The efficiency of in situ hybridization was found to range between 5 and 15% for both leukocyte and fibroblast cell types and for both metaphase and interphase nuclei. Determination of the parameters of the in situ hybridization reaction of ribosomal RNAs to diploid chromosomes define the experimental conditions needed for the localization of single copy genes to diploid chromosomes.
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