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Query: EC:2.3.1.28 (
chloramphenicol acetyltransferase
)
5,100
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
To define cis-acting genetic elements responsible for cell-specific transcriptional regulation of the
CC10
gene, DNA sequences spanning nucleotides -2338 to +49 of the rat
CC10
gene were linked to a reporter gene coding for
chloramphenicol acetyltransferase
(
CAT
). In transient expression assays,
CC10
sequences were capable of restricting
CAT
expression to a human lung adenocarcinoma cell line similar to pulmonary Clara cells. Transgenic mice harboring the hybrid RtCC10-
CAT
construct expressed high levels of
CAT
activity specifically within protein extracts of lung and trachea. Transcripts for the
CAT
reporter gene colocalized with those for the endogenous murine
CC10
gene within the airways of transgenic mice. Functional analysis of deletion mutants identified stimulatory, inhibitory, and cell type-specific transcriptional regulatory elements. The results of gel retention and DNaseI protection assays suggest that a transcriptional stimulatory region located between -320 and -175, and a cell type-specific regulatory element located between -175 and +49, result from a series of protein-DNA interactions occurring at -220 to -205 and -128 to -86, respectively. Lung epithelial specific transcriptional regulatory elements described herein will be useful for expression of chimeric genes within epithelial cells lining the trachea, bronchi, and bronchioles of mice.
...
PMID:cis-acting elements that confer lung epithelial cell expression of the CC10 gene. 163 15
Uteroglobin is expressed in various tissues of the rabbit under complex hormonal control. In the endometrium the
uteroglobin
gene is transcribed only in epithelial cells after administration of ovarian hormones. In this paper we demonstrate that within the promoter region of the rabbit
uteroglobin
gene, there is a functional estrogen-responsive element (ERE) located between -265 and -252. Hybrid constructions containing sequences of the
uteroglobin
promoter up to -299, linked to the
chloramphenicol acetyltransferase
gene of E. coli respond to estrogens in gene transfer experiments, whereas a deletion that removes half of the ERE does not. A synthetic oligonucleotide corresponding to the putative ERE is able to confer estrogen inducibility to an otherwise unresponsive promoter. Binding experiments with purified estrogen receptor from calf uterus reveal a DNase-I footprint over the ERE. Within this protected region six guanine residues that have been shown to be contacted by the receptor in other EREs are protected against methylation by dimethylsulfate in the presence of the estrogen receptor. We compare this ERE with the vitellogenin A2 ERE from Xenopus and find that the relative affinity of the
uteroglobin
ERE is slightly lower than that of the vitellogenin ERE. Thus, this
uteroglobin
ERE could be involved in physiological regulation of
uteroglobin
expression in the genital tract.
...
PMID:The uteroglobin promoter contains a noncanonical estrogen responsive element. 228 Jul 77
Transgenic animals bearing a chimeric gene containing 5'-flanking regions of the human surfactant protein C (SP-C) gene ligated to the bacterial
chloramphenicol acetyltransferase
(
CAT
) gene were analyzed by in situ hybridization histochemistry to determine the temporal and spatial distribution of transgene expression during organogenesis of the murine lung. Ontogenic expression of the SP-C-
CAT
gene was compared to that of the endogenous SP-C gene and to the Clara cell
CC10
gene. High levels of SP-C-
CAT
expression were observed as early as Day 10 of gestation in epithelial cells of the primordial lung buds. Low levels of endogenous SP-C mRNA were detected a day later, but only in the more distal epithelial cells of the newly formed, primitive, lobar bronchi. On Gestational Days 13 through 16, transcripts for both the endogenous and chimeric gene were restricted to distal epithelial elements of the branching bronchial tubules and were no longer detected in the more proximal regions of the bronchial tree. Although high levels of SP-C-
CAT
expression were maintained throughout organogenesis, endogenous SP-C expression increased dramatically on Gestational Day 15, coincident with acinar tubule differentiation at the lung periphery. Low levels of endogenous
CC10
expression were detected by Gestational Day 16 in both lobar and segmental bronchi. By the time of birth,
CC10
transcripts were expressed at high levels in the trachea and at all levels of the bronchial tree; endogenous SP-C mRNA was restricted to epithelial cells of the terminal alveolar saccules; and SP-C-
CAT
expression was now detected in both alveolar and bronchiolar epithelial cells. These results indicate that (1) cis-acting regulatory elements of the human SP-C gene can direct high levels of foreign gene expression to epithelial cells of the embryonic mouse lung; (2) expression of the human SP-C-
CAT
chimeric gene is developmentally regulated, exhibiting a morphogenic expression pattern similar, but not identical, to that of the endogenous murine SP-C gene; (3) the embryonic expression of endogenous SP-C and chimeric SP-C-
CAT
transcripts identifies progenitor cells of the distal respiratory epithelium; and (4) differentiation of bronchial epithelium is coincident with loss of SP-C expression and subsequent acquisition of
CC10
expression in proximal regions of the developing bronchial tubules.
...
PMID:Transcriptional elements from the human SP-C gene direct expression in the primordial respiratory epithelium of transgenic mice. 846 42
