Aso T scite author profile

Aso T

3Publications

374Citation Statements Received

17Citation Statements Given

How they've been cited

433

348

How they cite others

Affiliations

Tokyo Medical and Dental University, University of Fukui, Kyoto University

Publications

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Observation ofB±→pp¯
K¹,
R²,
Abe³
et al. 2002
Phys. Rev. Lett.
257
13
270
0
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We report the observation of the decay mode B(+/-) --> p(-)pK(+/-)based on an analysis of 29.4 fb(-1) of data collected by the Belle detector at KEKB. This is the first example of a b-->s transition with baryons in the final state. The p(-)p mass spectrum in this decay is inconsistent with phase space and is peaked at low mass. The branching fraction for this decay is measured to be B(B+/--->p(-)pK+/-) = [4.3(+1.1)(-0.9)(stat)+/-0.5(syst)]x 10(-6). We also report upper limits for the decays B(0)-->p(-)pK(S) and B(+/-)-->p(-)p pi(+/-).

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Characterization of cDNA for the large subunit of the transcription initiation factor TFIIF

Vasavada

Kawaguchi

et al. 1992

Nature

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At least six chromatographically resolvable general transcription factors may participate in accurate initiation by RNA polymerase II in HeLa cell-derived systems. TFIIF (also termed FC, RAP30/74 and beta/gamma) can bind directly to RNA polymerase II in solution and decrease the affinity of RNA polymerase II for nonspecific DNA. From studies on the kinetics of transcription initiation, on the composition of transcription initiation complexes fractionated by acrylamide gel electrophoresis, and on template competition experiments, TFIIF is known to act at an intermediate stage in initiation complex formation. It acts after TFIID firmly associates with DNA, but coincidentally with or immediately after RNA polymerase II binding to DNA, and before the recruitment of factor TFIIE. TFIIF may or may not have DNA helicase activity. The small subunit (RAP30) of TFIIF has been cloned and shows some amino-acid sequence homology to bacterial sigma factors. We have partially sequenced the RAP74 protein from purified HeLa cells, cloned its complementary DNA and shown that its translation product can interact with RAP30 in vitro as well as in vivo. The cDNA predicts an amino-acid sequence that lacks obvious DNA or RNA helicase motifs. It has regions rich in charged amino acids, including segments containing a higher content of acidic amino acids than are found in strong transcriptional activators such as VP16.

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Studies on the Pattern of Circulating Steroids in the Normal Menstrual Cycle

Guerrero¹,

T²,

Brenner³

et al. 1976

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In an attempt to analyze the multiple changes and interactions in cir¬ culating steroid levels in the peri-ovulatory and peri-menstrual periods, the plasma levels of immunoreactive luteinizing hormone (LH), pro¬ gesterone and unconjugated pregnenolone, dehydroepiandrosterone, testo¬ sterone, oestradiol and oestrone were assayed daily during a complete cycle in 17 normally menstruating women. In 14 of the 17 subjects studied androstenedione and unconjugated dihydrotestosterone were also esti¬ mated. The day of the LH-peak and the first day of menstruation, re¬ spectively, were used to synchronize the peri-ovulatory and peri-menstrual plasma levels of the various steroids.

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Aso T

Observation ofB±→pp¯
K¹,
R²,
Abe³
et al. 2002
Phys. Rev. Lett.
257
13
270
0
View full text Add to dashboard Cite

Characterization of cDNA for the large subunit of the transcription initiation factor TFIIF

Studies on the Pattern of Circulating Steroids in the Normal Menstrual Cycle

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Resources

About

Aso T

Observation ofB±→pp¯K1, R2, Abe3 et al. 2002Phys. Rev. Lett.257132700View full textAdd to dashboardCite

Characterization of cDNA for the large subunit of the transcription initiation factor TFIIF

Studies on the Pattern of Circulating Steroids in the Normal Menstrual Cycle

Contact Info

Product

Resources

About

Observation ofB±→pp¯
K¹,
R²,
Abe³
et al. 2002
Phys. Rev. Lett.
257
13
270
0
View full text Add to dashboard Cite