Yasuo Kikuchi scite author profile

From a cDNA library of mouse skeletal muscle, we have isolated mouse Sim1 (mSim1) cDNA encoding a polypeptide of 765 amino acids with striking amino acid identity in basic helix-loop-helix (89% identity) and PAS (89% identity) domains to previously identified mSim2, although the carboxy-terminal third of the molecule did not show any similarity to mSim2 or Drosophila Sim (dSim). Whole-mount in situ hybridization showed restricted and characteristic expression patterns of the two mSim mRNAs in various tissues and organs during embryogenesis, such as those for the somite, the nephrogenic cord, and the mesencephalon (for mSim1) and those for the diencephalon, branchial arches, and limbs (for mSim2). From sequence similarity and chromosomal localization, it is concluded that mSim2 is an ortholog of hSIM2, which is proposed to be a candidate gene responsible for Down's syndrome. The sites of mSim2 expression showed an overlap with the affected regions of the syndrome, further strengthening involvement of mSim2 in Down's syndrome.

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Possible function of Ah receptor nuclear translocator (Arnt) homodimer in transcriptional regulation.

Sogawa

Nakano

Kobayashi

et al. 1995

Proc. Natl. Acad. Sci. U.S.A.

174

118

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Synthesis of Poly-(l-prolyl-l-prolylglycyl) of Defined Molecular Weights

Sakakibara¹,

Kishida²,

Kikuchi³

et al. 1968

149

104

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A major problem in polypeptide synthesis is the formation of products with a wide range of molecular weights. As a step toward the total synthesis of natural protein, an attempt was made to synthesize a sequential polypeptide with a defined molecular weight. Thus, poly-(L-prolyl-L-prolylglycyl) with ten or twenty repeating units was synthesized by the step-by-step addition of AOC-L-prolyl-L-prolylglycine (I)1) using the solid-phase procedure.2) The synthesis was started from glycine-anchored polystyrene (100-200 mesh, copolymerized with 2% divinylbenzene; 14g, 0.1mmol/g), to which AOC-L-prolyl-L-proline (1.4g)1) was coupled in methylene chloride with dicyclohexylcarbodiimide. The AOCgroup was then removed with 2N hydrogen chloride in acetic acid, and the tripeptide-cycle was extended with I (1.7g per cycle) and dicyclohexylcarbodiimide (0.9g per cycle); each coupling reaction was carried out in methylene chloride for 3hr at room temperature. After nine reaction cycles, when ten repeating units were expected to have been formed, a part of the resin was dried (wt 7g) and placed in an HFreaction cylinder;3) anisole (7ml) was added, and then anhydrous hydrogen fluoride (HF, was introduced over the resin by means of the HFexcess HF was removed, and the peptide liberated was extracted with water. The water extract was treated with IR-45 (OH-form), and then dialyzed against distilled water for 3 days. The final solution was lyophilized (II, wt 0.

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Transactivation mechanisms of mouse clock transcription factors, mClock and mArnt3

et al. 2000

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A novel induction mechanism of the rat CYP1A2 gene mediated by Ah receptor–Arnt heterodimer

Sogawa

Numayama-Tsuruta

Takahashi

et al. 2004

Biochemical and Biophysical Research Communications

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Yasuo Kikuchi

Two New Members of the Murine Sim Gene Family Are Transcriptional Repressors and Show Different Expression Patterns during Mouse Embryogenesis

Possible function of Ah receptor nuclear translocator (Arnt) homodimer in transcriptional regulation.

Synthesis of Poly-(l-prolyl-l-prolylglycyl) of Defined Molecular Weights

Transactivation mechanisms of mouse clock transcription factors, mClock and mArnt3

A novel induction mechanism of the rat CYP1A2 gene mediated by Ah receptor–Arnt heterodimer

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