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Query: EC:2.4.2.7 (
adenine phosphoribosyltransferase
)
692
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
It has been documented that the activity of a specific promoter can be occluded by the presence of another promoter element upstream. We present evidence for a phenomenon contradictory to that predicted by the promoter occlusion theory. Transcription from the hamster
aprt
(
adenine phosphoribosyltransferase
) promoter was augmented instead of repressed in transfected mouse L cells when an upstream Moloney murine sarcoma virus enhancer-promoter element was induced with butyrate. Without an adjacent Moloney murine sarcoma virus element, butyrate could not activate the
aprt
promoter.
...
PMID:Transcriptional activation of the adenine phosphoribosyltransferase promoter by an upstream butyrate-induced Moloney murine sarcoma virus enhancer-promoter element. 215 51
The mouse
aprt
promoter contains four GC boxes, which bind transcription factor Spl in vitro, and lacks both TATA and CCAAT boxes. Removal of the two most distal GC boxes of this promoter had little effect on
APRT
enzyme levels produced in a transient expression assay. Deletion of the distal three GC boxes resulted in a 50% reduction, and deletion of all GC boxes resulted in essentially complete loss of
APRT
activity. There are two predominant transcription start sites which are located within the region containing the GC boxes. The promoter behaved as a relatively strong promoter when compared to the RSV LTR promoter in a transient CAT assay, and operated in one orientation only. No upstream anti-sense transcripts were detected in either mouse CAK or liver cells, confirming that the mouse
aprt
promoter, unlike some other GC-rich promoters appears not to support bidirectional transcription.
...
PMID:Identification of DNA sequences required for mouse APRT gene expression. 290 25
DNA-mediated gene transformation of mouse Ltk-
aprt
-hprt-cells was used to obtain stable, doubly selected transformants simultaneously expressing herpes virus thymidine kinase (TK) and mammalian
adenine phosphoribosyltransferase
(
APRT
). Cotransformants occurred at a frequency of 5 X 10(-6), a similar frequency for the transfer of the
aprt
marker has been previously observed. Isozyme and Southern blot analysis show that the TK and
APRT
expressed in these transformants resulted from gene transfer. For one stable cotransformant, [3H]thymidine [( 3H]TdR) selection against TK activity resulted in the loss of
APRT
activity as well, suggesting that these genes had become genetically linked together. Similarly selection against
APRT
expression resulted in the loss of a subset of the transferred herpes simplex virus tk genes. 5-Bromodeoxyuridine (BUdR) selected TK- variants differed from [3H]TdR selected TK- variants, in that they retained tk genes. However, BUdR-selected variants expressed full levels of
APRT
. Therefore, even though the transferred tk and
aprt
genes had become genetically linked together, they were, in this case, independently expressed since these cells were phenotypically TK- and APRT+.
...
PMID:Genetic linkage but independent expression of functional HSV-1 tk and mammalian aprt genes after cotransfer to L cells. 298 26
The 5' end of the Chinese hamster ovary
aprt
gene was sequenced and transcription start sites were determined by both S1 nuclease protection and primer extension assays. Deletion mutants covering the same area were constructed, and
adenine phosphoribosyltransferase
(
APRT
) or chloramphenicol acetyltransferase (CAT) activity was measured by transient-expression assays. The
aprt
gene uses a single cluster of transcription start sites and lacks consensus sequences such as TATA and CCAAT, which are general components of eucaryotic promoters. The 5' deletion mutations of the promoter sequences demonstrated that (i) there is no decrease in either
APRT
activity or transcription extending to position -89 (relative to the main transcription start site); (ii) an additional 29-base-pair (bp) deletion decreases
APRT
activity and transcription twofold; and (iii) a deletion past the transcription start sites (P5' delta +27) abolishes both
APRT
activity and transcription, indicating that a 60-bp fragment immediately upstream of the main transcription start site is involved in basic transcription and a 29-bp fragment just upstream of the 60 bp-fragment stimulates transcription twofold. The 3' deletion mutations showed that a deletion of a 61-bp fragment in the 5' leader and coding sequence abolishes the efficient translation of an
aprt
-CAT gene transcript. In addition, there are two polyadenylation signals at the genomic 3' end, with the proximal one being sufficient for functional polyadenylation.
...
PMID:Analysis of signals controlling expression of the Chinese hamster ovary aprt gene. 340 12
A series of mouse-human hybrids was prepared from mouse cells deficient in
adenine phosphoribosyltransferase
(
EC 2.4.2.7
) and normal human cells. The hybrids were made in medium containing adenine and alanosine, an antimetabolite known to inhibit de novo adenylic acid biosynthesis. The mouse cells, unable to utilize exogenous adenine, were killed in this medium, but the hybrids proliferated as a consequence of their retaining the human
aprt
gene. The hybrids were then exposed to the adenine analogs 2,6-diaminopurine and 2-fluoroadenine to select for cells that had lost this gene. Before exposure to the adenine analogs, the expression of human
adenine phosphoribosyltransferase
by the hybrids was strongly associated only with the presence of human chromosome 16, and afterwards this was the only human chromosome consistently lost. This observation suggests that the human
aprt
gene can be assigned to chromosome 16.
...
PMID:Assignment of the gene for adenine phosphoribosyltransferase to human chromosome 16 by mouse-human somatic cell hybridization. 412 2
A system that selects for the gene directing synthesis of the enzyme
adenine phosphoribosyltransferase
(
APRT
) uses the antibiotic alanosine to prevent endogenous synthesis of adenylic acid. With the aid of this system, a new series of human-mouse hybrids has been prepared between wild type human diploid fibroblasts and an enzyme-deficient mouse line. Survival of the hybrids depended upon the presence of the
APRT
, which was shown to have the isoelectric pH characteristic of the human enzyme and not that of the mouse. Reduced hybrids containing the enzyme lacked all human biarmed chromosomes, so that unless a rearrangement had occurred, the
aprt
gene must be located on an acrocentric chromosome. The hybrid cells became
APRT
(-) with a frequency of 2 x 10(-3), probably by loss of the human
aprt
chromosome. The
APRT
(-) progeny could be obtained selectively by growth in medium containing fluoroadenine.
...
PMID:A new reduced human-mouse somatic cell hybrid containing the human gene for adenine phosphoribosyltransferase. 527 4
Evidence for a two-step model to explain the high-frequency expression of the recessive phenotype at the autosomal
adenine phosphoribosyltransferase
(
APRT
;
EC 2.4.2.7
) locus in Chinese hamster ovary (CHO) cells was given by Simon et al. [Simon, A. E., Taylor, M. W., Bradley, W. E. C. & Thompson, L. (1982) Mol. Cell. Biol. 2, 1126-1133]. This model proposed a high-frequency event, leading to allelic inactivation or a loss of gene function, and a low-frequency event, causing a structural alteration of the
APRT
protein. Either event could occur first, resulting in two classes of heterozygotes. We have analyzed the low-frequency event that gave rise to the class 2
aprt
heterozygote D416 and the high-frequency event that led to
APRT
- cells derived from D416. Genomic Southern blots of Msp I- or Hpa II-digested DNA from wild-type CHO,
aprt
heterozygote D416, and two
APRT
- cell lines derived from D416 indicate a loss of a specific Msp I/Hpa II recognition sequence at one
aprt
locus in the heterozygote that correlates with the production of the electrophoretically altered
APRT
protein found in D416. The
APRT
- mutants are homozygous for the loss of this Msp I/Hpa II site. By using an additional CHO gene as an internal control, it was determined that the
APRT
- mutants contain only a single copy of the altered
aprt
gene. Thus, the high-frequency event that produces
APRT
- mutants derived from D416 is not an inactivation event but rather a deletion of the wild-type
aprt
gene.
...
PMID:High-frequency mutation at the adenine phosphoribosyltransferase locus in Chinese hamster ovary cells due to deletion of the gene. 657 71
The potent tumor promoter 12-O-tetradecanoylphorbol-13-acetate (TPA) was tested for its ability (a) to induce sister chromatid exchange, (b) to increase the rate of transition at the
adenine phosphoribosyltransferase
(apt) locus from the presumptive heterozygous state ((+/- to the homozygous state (-/ - or -), and (c) to enhance the frequency of mutations expressed after ultraviolet radiation mutagenesis. We have found no significant effect of TPA in any of these experiments. Sister chromatid exchange frequencies in both V79 and Chinese hamster ovary cells remained unchanged by TPA treatment under various conditions, a result inconsistent with the hypothesis that an important effect of TPA might be to increase the rate of chromosomal mitotic recombination (and hence segregation of recessive mutations) in a manner akin to increased chromatid recombination. We have also been unable to obtain evidence for mitotic recombination affecting the
aprt
locus in Chinese hamster ovary cells for which the rate of change to a high level of resistance to azaadenine was measured. The rate of 8.6 X 10(-7) mutation (and/or segregations) per cell generation assessed by fluctuation analysis was not increased by the continuous presence of TPA, 4 microgram/ml, in the medium. In the third set of experiments, mutant frequencies in Chinese hamster ovary cells after ultraviolet mutagenesis were measured for the markers ouabain resistance, thioguanine resistance, and azaadenine resistance, under conditions with and without pretreatment with TPA before mutant selection. No convincing enhancement in mutation expression was observed. In summary, these results argue that promotion by TPA does not proceed by a mechanism involving genetic recombination or the altered expression of newly mutated alleles.
...
PMID:Failure of the phorbol ester 12-O-tetradecanoylphorbol-13-acetate to enhance sister chromatid exchange, mitotic segregation, or expression of mutations in Chinese hamster cells. 693 1
Conditions for reliable and efficient assay of mutations affecting the activity of HPRT (hypoxanthine phosphoribosyltransferase EC 2.4.2.8) and
APRT
(
adenine phosphoribosyltransferase
EC 2.4.2.7
) have been determined for a strain of CHO (Chinese hamster ovary) cells that has been adapted for rapid growth both in suspension culture and in monolayer. To facilitate measurement of mutation at the
aprt
locus, clones were derived that are presumptively heterozygous at that locus. At a limiting concentration of 8 microgram/ml of azaadenine, 14/16 of the resistant clones picked and tested had approximately 1/2 of the
APRT
activity of the wild-type cells. One such clone, strain AA8, was chosen for further studies and found to be readily mutable to resistance to 80 microgram/ml azaadenine. Most of the highly resistant colonies isolated (21/24) had very low in vitro
APRT
activity. The optimal conditions for detection of TGr and AAr mutations were determined for two critical parameters, expression time and cell density. Cultures treated with mutagen either in monolayer or in suspension were allowed to express mutations in suspension. The expression of mutations induced by UV light, EMS, and ICR-191 was complete by 3 days for AAr and by 4-5 days for TGr. The time required to reach a maximal frequency of mutants was essentially independent of the type of mutagen and the level of survival after treatment. Induced mutation frequencies for both loci were notably stable during the time intervals examined. With respect to cell-density conditions, both markers were detected at frequencies that were independent of the cell inocula over the range of 1 x 10(5) to 1 x 10(6) cells per 100-mm petri dish (i.e. 1.6 x 10(3) to 1.6 x 10(4) cells/cm2) containing 20 ml of medium. These results were obtained with both mutagenized populations and with reconstructed mixtures obtained by adding drug-resistant cells to varying numbers of wild-type cells. The rapid expression of mutations for both markers, particularly AAr, combined with the advantage that large inocula can be plated for selection of mutants, make this CHO strain an attractive system for the simultaneous measurement of mutations at the autosomal
aprt
and X-linked hprt loci.
...
PMID:Validation of conditions for efficient detection of HPRT and APRT mutations in suspension-cultured Chinese hamster ovary cells. 736 Jan 55
The
aprt
locus in TK6 human lymphoblasts has been previously shown to have an unusual mutation frequency (5 x 10(-8) and a gene dosage of 2. Measurements of mutation rate (1.2 x 10(-9)) reported here, confirm the mutation-frequency observations. These results are not easily accommodated by models of the gene as functionally homozygous or heterozygous. Characterization of all exon and intron sequences identified no polymorphism which could distinguish two heterozygous
aprt
alleles. Furthermore, autoradiographs of 16 spontaneous
APRT
- mutants demonstrate a variety of unique sequences. If
aprt
were heterozygous, wild-type sequence from the alternate allele would be observed at positions where mutations have occurred. These observations cannot be explained by conventional loss of heterozygosity in which the same mutated allele would be repeatedly recovered. We therefore propose that
aprt
is a functionally homozygous locus.
APRT
- mutants may arise by conventional mutation of one allele, and high-frequency loss or conversion of the alternate allele.
...
PMID:Evidence for high-frequency allele loss at the aprt locus in TK6 human lymphoblasts. 769 Aug 93
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