Abnormal fertility, acrosome formation, IFT20 expression and localization in conditional Gmap210 knockout mice

Author:

Wang Zhenyu12,Shi Yuqin1,Ma Suheng12,Huang Qian12,Yap Yi Tian2,Shi Lin12,Zhang Shiyang12,Zhou Ting12,Li Wei2,Hu Bo3,Zhang Ling1,Krawetz Stephen A.4,Pazour Gregory J.5,Hess Rex A.6,Zhang Zhibing24

Affiliation:

1. School of Medicine, Hubei Province Key Laboratory of Occupational Hazard Identification and Control, Wuhan University of Science and Technology, Wuhan, China

2. Department of Physiology, Wayne State University, Detroit, Michigan

3. Department of Neurology, Wayne State University, Detroit, Michigan

4. Department of Obstetrics/Gynecology and Center for Molecular Medicine and Genetics, Wayne State University, Detroit, Michigan

5. Program in Molecular Medicine, University of Massachusetts Medical School, Worcester, Massachusetts

6. Department of Comparative Biosciences, College of Veterinary Medicine, University of Illinois, Urbana, Illinois

Abstract

GMAP210 (TRIP11) is a cis-Golgi network-associated protein and a Golgi membrane receptor for IFT20, an intraflagellar transport component essential for male fertility and spermiogenesis in mice. To investigate the role of GMAP210 in male fertility and spermatogenesis, floxed Gmap210 mice were bred with Stra8-iCre mice so that the Gmap210 gene is disrupted in spermatocytes and spermatids in this study. The Gmap210flox/flox: Stra8-iCre mutant mice showed no gross abnormalities and survived to adulthood. In adult males, testis and body weights showed no difference between controls and mutant mice. Low-magnification histological examination of the testes revealed normal seminiferous tubule structure, but sperm counts and fertility were significantly reduced in mutant mice compared with controls. Higher resolution examination of the mutant seminiferous epithelium showed that nearly all sperm had more oblong, abnormally shaped heads, while the sperm tails appeared to have normal morphology. Electron microscopy also revealed abnormally shaped sperm heads but normal axoneme core structure; some sperm showed membrane defects in the midpiece. In mutant mice, expression levels of IFT20 and other selective acrosomal proteins were significantly reduced, and their localization was also affected. Peanut-lectin, an acrosome maker, was almost absent in the spermatids and epididymal sperm. Mitochondrion staining was highly concentrated in the heads of sperm, suggesting that the midpieces were coiling around or aggregating near the heads. Defects in acrosome biogenesis were further confirmed by electron microscopy. Collectively, our findings suggest that GMAP210 is essential for acrosome biogenesis, normal mitochondrial sheath formation, and male fertility, and it determines expression levels and acrosomal localization of IFT20 and other acrosomal proteins.

Funder

NIH

Start up fund of wayne state university

start up fund of wayne state university

National Natural Science Foundation of China

Excellent youth foundation of hubei science and technology office

Youth foundation of hubei science and technology office

The China Scholarship Council Fund

Publisher

American Physiological Society

Subject

Cell Biology,Physiology

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