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FUNCTIONAL ANALYSIS OF CA/CALMODULIN-DEPENDENT PROTEIN KINASE II IN PANCREATIC BETS-CELLS WITH CONDITIONAL KNOCKOUT MICE.

Research Project

Project/Area Number 15590949
Research Category

Grant-in-Aid for Scientific Research (C)

Allocation TypeSingle-year Grants
Section一般
Research Field Metabolomics
Research InstitutionKUMAMOTO UNIVERSITY

Principal Investigator

MATSUMOTO Kazuya  KUMAMOTO UNIVERSITY HOSPITAL, METABOLISM and ENDOCRINOLOGY, RESEARCH ASSISTANT, 医学部附属病院, 助手 (80346999)

Co-Investigator(Kenkyū-buntansha) MIYAMURA Nobuhiro  KUMAMOTO UNIVERSITY HOSPITAL, METABOLISM and ENDOCRINOLOGY, LECTURER, 医学部附属病院, 講師 (40274716)
TOYONAGA Tetsushi  KUMAMOTO UNIVERSITY, GRADUATE SCHOOL OF MEDICAL SCIENCE, METABOLIC MEDICINE, RESEARCH ASSISTANT, 大学院・医学薬学研究部, 助手 (60295128)
ARAKI Eiichi  KUMAMOTO UNIVERSITY, GRADUATE SCHOOL OF MEDICAL SCIENCE, METABOLIC MEDICINE, PROFESSOR, 大学院・医学薬学研究部, 教授 (10253733)
Project Period (FY) 2003 – 2004
Project Status Completed (Fiscal Year 2004)
Budget Amount *help
¥3,600,000 (Direct Cost: ¥3,600,000)
Fiscal Year 2004: ¥1,100,000 (Direct Cost: ¥1,100,000)
Fiscal Year 2003: ¥2,500,000 (Direct Cost: ¥2,500,000)
KeywordsPANCREATIC BETA CELLS / CALCIUM / CALMODULIN / INSULIN SECRETION / KNOCKOUT MOUSE / PROMOTER ANALYSIS / INHIBITORY PROTEIN / Cre recombinase
Research Abstract

We have reported that Ca/calmodulin-dependent protein kinase II(CaM kinase II) was involved in insulin secretion. The aim of this study is to further analyze the roles of CaM kinase II in pancreatic beta cells. The 19 kb genomic clone of CaM kinase II delta subunit was isolated from C57/BL6 mouse genomic library and ascertained to contain the exon that encoded initial codon. Restriction enzyme sites were analyzed and three unique restriction enzyme sites were identified at upsteam(Nae I) or downstream(Sex AI, Pfl MI) of the exon. A lox P fragment was amplified, attached by Nae I recognition sequences in both ends and inserted into Nae I site of the clone. Furthermore, thymidine kinase cDNA attached by lox P and Sex AI sequence and diphtheria toxin B cDNA were planned to insert the clone to construct targeting vector. Also endogenous inhibitory peptide for CaM kinase II(CaM KIIN) cDNA was isolated from MIN6 cells. Adenoviral expression vector of CaM KIIN was preparing to analyze the role of CaM kinase II in beta cells. Moreover, promoter region of the CaM kinase II delta subunit gene was analyzed with luciferase reporter gene. The 2.1 kb upstream region from TATA-like sequence seemed to contain promoter activity. Possible transcriptional factor binding sites were identified in the region.

Report

(3 results)
  • 2004 Annual Research Report   Final Research Report Summary
  • 2003 Annual Research Report
  • Research Products

    (4 results)

All 2005 2004

All Journal Article (4 results)

  • [Journal Article] AICAR, an activator of AMP-activated protein kinase, down-regulates the insulin receptor expression in HepG2 cells2005

    • Author(s)
      Nakamaru K, Matsumoto K, et al.
    • Journal Title

      Biochem.Biophy Res Commun 328

      Pages: 449-454

    • Related Report
      2004 Annual Research Report
  • [Journal Article] Enhanced expression of PDX-1 and Ngn3 by exendin-4 during β cell regeneration in STZ-treated mice2005

    • Author(s)
      Kodama S, Yoyonaga T, Kon-do T, Matsumoto K, et al.
    • Journal Title

      Biochem.Biophy Res Commun 327

      Pages: 1170-1178

    • Related Report
      2004 Annual Research Report
  • [Journal Article] 感音性難聴を伴うBartter症候群の1例-barttin遺伝子異常による新しい病型2004

    • Author(s)
      宮村信博, 松本和也, 他
    • Journal Title

      ホルモンと臨床 52

      Pages: 152-158

    • NAID

      10013547563

    • Related Report
      2004 Annual Research Report
  • [Journal Article] 糖尿病における膵臓の役割2004

    • Author(s)
      松本和也, 荒木栄一
    • Journal Title

      Mebio 21

      Pages: 28-36

    • Related Report
      2004 Annual Research Report

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Published: 2003-04-01   Modified: 2016-04-21  

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