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Molecular and cellular biological mechanism of the deteriorated spermatogenesis : analysis of glycoprotein in basal membrane of seminiferous tubules.

Research Project

Project/Area Number 15591719
Research Category

Grant-in-Aid for Scientific Research (C)

Allocation TypeSingle-year Grants
Section一般
Research Field Urology
Research InstitutionSt.Marianna University School of Medicine

Principal Investigator

IWAMOTO Teruaki  St.Marianna University School of Medicine, Dept. of Urology, Director, 医学部, 教授 (60046117)

Co-Investigator(Kenkyū-buntansha) SATOH Yoko  Japan Science and Technology Agency, Researcher, 研究員
Project Period (FY) 2003 – 2004
Project Status Completed (Fiscal Year 2004)
Budget Amount *help
¥3,400,000 (Direct Cost: ¥3,400,000)
Fiscal Year 2004: ¥1,600,000 (Direct Cost: ¥1,600,000)
Fiscal Year 2003: ¥1,800,000 (Direct Cost: ¥1,800,000)
Keywordsspermatogenesis / lamina propria / glycoprotein / progesterone / cell line / testis
Research Abstract

Thickened lamina propria in seminiferous tubules of the testis is unique morphological feature of human testis showing deteriorated spermatogenesis. Previously, we showed that inner layer of thickened lamina propria had glycoproteins recognized by PNA-lectin and included progesterone detected by antiprogesterone antibody. However, there was no other information about the product of the inner layer of lamina propria. To clarify the role of lamina propria in spermatogenesis, we need to identify products which are increased in the inner layer. Combining information about the cells and lamina propria in testis by immunohistochemistry, we developed a screening method of isolating glycoproteins recognized by PNA-lectin. Testicular samples from a patient showing almost normal spermatogenesis and a patient showing deteriorated spermatogenesis were homogenized and solubilized. The solubilized proteins were analyzed by 2-D gel electrophoresis. The positive spots by PNA-lectin affinity blotting a … More nd negative spots by collagen IV and vimentin V9 Ab western blotting were screened. One of the spots was M.W. 43kDa with a pI of 5-6 and was thought to be a novel albumin like protein from the results by LC-MS/MS and MASCOT search. However, this screening method was insufficient to determine the concerned glycoproteins in lamina propria and additional informations were needed. After investigation of binding substances to the thickened lamina propria, thickened lamina propria showed the property to bind progesterone and this glycoprotein also could bind to progesterone. We continues the analysis of the glycoproteins by new method contained the additional steps for properties of glycoproteins. As another projects, we tried to establish the immortalized cell line derived from human testis to investigate the synthesis of glycoproteins under cellular level. First, primary cultured testicular cells showing better growth were selected and then examined the efficiency of transfection using EGFP as a marker. We found that anti-infectous virus vector is optimum for our needs. Less

Report

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

    (3 results)

All 2003 Other

All Journal Article (2 results) Publications (1 results)

  • [Journal Article] Male reproductive health and effect of endocrine disruptors.2003

    • Author(s)
      Iwamoto T, Sato Y, Nozawa S
    • Journal Title

      Env. Sci. 10

      Pages: 1-12

    • Description
      「研究成果報告書概要(和文)」より
    • Related Report
      2004 Final Research Report Summary
  • [Journal Article] Male reproductive health and effect of endocrine disruptors.2003

    • Author(s)
      Iwamoto T, Sato Y, Nozawa S
    • Journal Title

      Env.Sci. 10

      Pages: 1-12

    • Description
      「研究成果報告書概要(欧文)」より
    • Related Report
      2004 Final Research Report Summary
  • [Publications] Iwamoto T: "Male reproductive health and effect of endocrine disruptors."Env.Sci.. 10. 1-12 (2003)

    • Related Report
      2003 Annual Research Report

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

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