Gene/Protein
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Enzyme
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Gene/Protein
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Target Concepts:
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Query: EC:3.1.31.1 (
micrococcal nuclease
)
2,818
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
In situ hybridization revealed an apparently higher expression of N-ras and
c-fos
in human hepatoma than in its adjacent liver tissue. When the isolated nuclei were partially digested with
micrococcal nuclease
followed by DNA extraction, gel electrophoresis and hybridization with labelled probes, it was shown that in hepatoma the
c-fos
and N-ras DNA sequences were mainly distributed on the nucleosomes of lower order structures, while these gene sequences in the adjacent liver tissue were found mainly on the nucleosomes of higher order structures. These results clearly indicate a close correlation between gene expression and chromatin conformation of
c-fos
and N-ras.
...
PMID:Correlation between gene expression and chromatin conformation of c-fos and N-ras in human liver and hepatoma. 166 52
Androgen receptors were quantified in nuclei from human prostate tissue and in nuclear fractions derived by exhaustive digestion with
micrococcal nuclease
. In nuclei from benign hypertrophic prostate (BPH), the population of androgen receptors solubilized during nucleolysis predominated whereas in carcinoma nuclei the nuclease-resistant population was in excess. This phenomenon was restricted to intranuclear deployment and could not be attributed to recompartmentalization within the cell. Receptor content could not be correlated to the expression of the cellular protooncogenes myc, H-ras, K-ras or sis, in either BPH or carcinoma. However, in both BPH and carcinoma, significant correlation was observed between nuclear androgen receptor content and expression of
c-fos
. Expression of
c-fos
was not elevated in carcinoma compared to BPH, whereas expression of c-myc was elevated in carcinoma specimens of all grades of glandular differentiation, and expression of H-ras became increasingly elevated as differentiation was lost.
...
PMID:Intranuclear androgen receptor deployment and protooncogene expression in human diseased prostate. 244 4
A procedure for the isolation of transcriptionally active nucleosomes was used to monitor changes in chromatin structure during the activation, repression, and superinduction of the protooncogenes
c-fos
and c-myc. Nuclei were isolated from murine fibroblasts at successive times after stimulation of quiescent cell cultures with serum or platelet-derived growth factor. The nucleosomes released by a brief
micrococcal nuclease
digestion were fractionated by HgII-affinity chromatography to separate the unfolded nucleosomes of transcriptionally active genes (in which the sulfhydryl groups of histone H3 are accessible for binding to HgII) from the compactly beaded nucleosomes of transcriptionally inert DNA sequences (in which the H3 sulfhydryl groups are not accessible). The DNA sequence contents of the HgII-bound and unbound nucleosome fractions were compared by slot-blot hybridizations to 32P-labeled cloned probes for
c-fos
and c-myc. The binding of the
c-fos
and c-myc nucleosomes to the HgII column accurately reflected both the timing and the degree of their expression, as determined by run-off transcription assays with the isolated nuclei. The superinduction of
c-fos
and c-myc expression by an inhibitor of protein synthesis (cycloheximide) was reflected in the persistence of the unfolded, transcriptionally active state of their component nucleosomes. These results provide direct evidence that rapid and reversible changes in nucleosome topography accompany the program of oncogene expression, and they suggest a way to monitor aberrant gene activity during malignant transformation.
...
PMID:Rapid and reversible changes in nucleosome structure accompany the activation, repression, and superinduction of murine fibroblast protooncogenes c-fos and c-myc. 347 51
Human promyelocytic leukemic (HL-60) cells have amplified c-myc protooncogene sequences which lead to an elevated level of c-myc gene expression. Induction of HL-60 cells by phorbol esters to undergo monocytic differentiation results in the suppression of c-myc, but the activation of
c-fos
gene transcription. Chromatin structures of c-myc and
c-fos
were compared by measuring their sequences in nucleosome-associated DNA fragments. These nucleosomal particles were released from chromatin by
micrococcal nuclease
digestion and subsequently analyzed with two dimensional gel electrophoresis. C-myc related sequences were detected in nucleosomal DNA fragments of differentiated cells only, while the
c-fos
related sequences were found in nucleosomal DNAs of noninduced HL-60 cells. Since the enzyme preferentially digests relaxed DNAs, these results suggest that nucleosomal subunits of c-myc and
c-fos
chromatin are relaxed during the state of active transcription, and reassembled once their transcription is repressed.
...
PMID:Reassembly of c-myc and relaxation of c-fos nucleosomes during differentiation of human leukemic (HL-60) cells. 354 26
