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2School of Biology, Lomonosov Moscow State University, Moscow 119992, Russia; fax: (095) 939-4309; E-mail: smirnov_an@hotmail.com
* To whom correspondence should be addressed.
Received February 4, 2002; Revision received February 22, 2002
Using electromobility shift assay the interaction of fragments of two paralogous rat estrogen sulfotransferase (Ste) genes with proteins of nuclear extracts from male and female rat liver was studied. Male-specific DNA-protein complexes were revealed with labeled oligonucleotides corresponding to fragments +1150/+1449, +1358/+1449, +1397/+1449, and +1417/+1449 of intron 1 of the Ste1 gene. The removal of a 20 bp region corresponding to the sequence +1430/+1449, or even either 5´- or 3´-terminal 5 bp of this region abolished the selective interaction of the oligonucleotides with the male-specific protein(s). According to the results of the experiments on mutual competition of the oligonucleotides, the fragment of the Ste2 gene corresponding to the sequence +1397/+1449 of the Ste1 gene formed complexes with the same male-specific protein(s) as the fragment of the Ste1 gene did. The data suggest the mapped element to participate in gender differentiation of the expression of the Ste1 and Ste2 genes.
KEY WORDS: estrogen sulfotransferase, sex differentiation, gene expression, regulatory elements, DNA-protein interaction, liver
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