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(Received for publication, September 1,
1995; and in revised form, October 31, 1995) H1t is synthesized in mid to late pachytene spermatocytes of the
male germ line and is the only tissue-specific member of the mammalian
H1 histone family. As a step toward identifying DNA sequences that
confer its tissue-specific expression, we have produced transgenic mice
containing the intact rat H1t gene as well as a H1t-lacZ
fusion gene. Transgenic mice carrying a 6.8-kilobase fragment of rat
genomic DNA encompassing the H1t gene expressed rat H1t at high levels
in the testis and in no other organ examined. H1t fragments truncated
to within 141 base pairs (bp) of the gene in the 5` direction or within
837 bp in the 3` direction retained testis specificity. Expression of
rat H1t protein was also evident in the testes of the transgenic mice,
and in some lines the level of rat H1t exceeded that of the mouse
protein. The stage of spermatogenesis of transgene expression was
assessed by following appearance of transgenic mRNA in developing mice
and by immunohistochemistry using an antiserum to rat H1t. In lines
from three different constructs, expression was restricted to germinal
cells, although in two strongly expressing lines the transgenes were
expressed somewhat prematurely in preleptotene spermatocytes. An
H1t(-948/+71)-lacZ fusion was also expressed
specifically in the spermatocytes and round spermatids of a transgenic
line, confirming that sequences sufficient for correct tissue and
developmental expression lie within this 1,019-bp segment of the gene.
Volume 271,
Number 8,
Issue of February 23, 1996 pp. 4046-4054
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
ONE KILOBASE OF 5`-FLANKING SEQUENCE MEDIATES CORRECT EXPRESSION OF
A lacZ FUSION GENE
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