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Enzyme
Compound
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Target Concepts:
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Query: EC:3.2.1.23 (
beta-galactosidase
)
14,648
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
We investigated the role of sequences flanking the transcription initiation site of the delta 1-
crystallin
gene in transient transfection assays of primary embryonic chicken lens epithelial cells or fibroblasts. Varying lengths of the 5' flanking sequence of the delta 1-
crystallin
gene (containing some untranslated sequence from exon 1) were fused to the bacterial chloramphenicol acetyltransferase (CAT) gene in the pSVOCAT plasmid. A plasmid carrying the bacterial
beta-galactosidase
gene driven by the Rous sarcoma virus (RSV) promoter was used as an internal control. Standardized results showed that the sequence located between -120 to -43 exhibited strong promoter activity; however, the promoter activity was markedly reduced (20-fold) when the upstream sequence between -603 and -120 was included in the construct. The delta 1-
crystallin
promoter displayed little lens preference. This upstream sequence did not reduce the activity of the Simian virus 40 (SV40) early promoter (with or without its enhancer) or the Herpes thymidine kinase promoter in transfection tests, indicating some specificity in its effect. Evidence for a delta 1-
crystallin
negative trans-acting factor was provided by competition experiments. Our data raise the possibility that expression of the delta 1-
crystallin
gene involves a negative cis-acting transcription element, a speculation which may deserve further attention in view of the gradual decrease in delta-
crystallin
synthesis in the developing lens.
...
PMID:Evidence for positive and negative regulation in the promoter of the chicken delta 1-crystallin gene. 283 46
Transgenic mice carrying the gamma 2-
crystallin
promoter fused to the coding region of the bacterial lacZ gene were generated. The offspring of three founder mice expressed high levels of the enzyme solely in the central nuclear fiber cells of the lens as measured by an in situ assay for the detection of
beta-galactosidase
activity. These results suggest that gamma 2-
crystallin
sequences between -759 to +45 contain essential information required for appropriate tissue-specific and temporal regulation of the mouse gamma 2-
crystallin
gene. In a broader context, this study also demonstrates the utility of
beta-galactosidase
hybrid gene constructs for monitoring the activity of gene regulatory elements in transgenic mice.
...
PMID:In situ detection of beta-galactosidase in lenses of transgenic mice with a gamma-crystallin/lacZ gene. 309 90
The small heat-shock proteins (sHsp), including Hsp27 and alphaB-
crystallin
, usually form large oligomers in cells. It has been suggested that the sHsp form oligomers by binding either a conserved C-terminal amino acid sequence or the less conserved N-terminal region. However, the site of binding has not been precisely determined. We used the yeast two-hybrid system to investigate binding of full-length rat Hsp27 or fragments of Hsp27 to full-length rat Hsp27 or alphaB-
crystallin
molecules. A series of cDNAs coding for fragments of Hsp27 were generated and ligated with the coding sequence for the binding domain of the yeast Gal4p transcription factor. These cDNAs were each transfected into yeast that had been transfected to express full-length rat Hsp27 or alphaB-
crystallin
fused with the DNA binding domain of Gal4p. Yeast cells transfected with both plasmids were assayed, by both a
beta-galactosidase
(beta-gal) filter assay and a quantitative liquid assay, for activation of Gal4p-driven beta-gal expression. Results indicated that the N-terminal domain of Hsp27 consisting of amino acids 1-124 did not bind to Hsp27 or alphaB-
crystallin
. The predominant Hsp27-Hsp27/alphaB-
crystallin
binding domain was the conserved C-terminal region consisting of amino acids 141-206, particularly amino acids 141-176.
...
PMID:Identification of a site of Hsp27 binding with Hsp27 and alpha B-crystallin as indicated by the yeast two-hybrid system. 1004 95
To elucidate the regulatory mechanisms underlying lens development, we searched for members of the large Maf family, which are expressed in the mouse lens, and found three, c-Maf, MafB, and Nrl. Of these, the earliest factor expressed in the lens was c-Maf. The expression of c-Maf was most prominent in lens fiber cells and persisted throughout lens development. To examine the functional contribution of c-Maf to lens development, we isolated genomic clones encompassing the murine c-maf gene and carried out its targeted disruption. Insertion of the
beta-galactosidase
(lacZ) gene into the c-maf locus allowed visualization of c-Maf accumulation in heterozygous mutant mice by staining for LacZ activity. Homozygous mutant embryos and newborns lacked normal lenses. Histological examination of these mice revealed defective differentiation of lens fiber cells. The expression of
crystallin
genes was severely impaired in the c-maf-null mutant mouse lens. These results demonstrate that c-Maf is an indispensable regulator of lens differentiation during murine development.
...
PMID:Regulation of lens fiber cell differentiation by transcription factor c-Maf. 1038 33
