Abstract
Densitometric analysis has been performed on mouse chromosomes from "in vivo" preparations stained with Giemsa after trypsinisation. The characteristic curves obtained by analysing the same chromosome after different durations of trypsinisation suggest that a trypsinisation step is not always necessary to get an analysable banding pattern. The best results are obtained when the chromatids are long and closely appressed and by analysing the positive photomicrographs.
Publisher
Canadian Science Publishing
Subject
Cell Biology,Plant Science,Genetics
Cited by
5 articles.
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