4.4 Article

Three male germline-specific aldolase A isozymes are generated by alternative splicing and retrotransposition

Journal

DEVELOPMENTAL BIOLOGY
Volume 309, Issue 1, Pages 18-31

Publisher

ACADEMIC PRESS INC ELSEVIER SCIENCE
DOI: 10.1016/j.ydbio.2007.06.010

Keywords

spermatogenesis; sperm; glycolysis; aldolase isozymes; retrogene; retrotransposition; alternative splicing; fibrous sheath; LC-MALDI-MS

Funding

  1. NICHD NIH HHS [U54 HD035041-115746, U54 HD35041, U54 HD035041] Funding Source: Medline
  2. NIGMS NIH HHS [P50 GM076468-01, P50 GM076468, 1P50 GM076468] Funding Source: Medline

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Enzymes in the glycolytic pathway of mammalian sperm are modified extensively and are localized in the flagellum, where several are tightly bound to the fibrous sheath. This study provides the first evidence for three novel aldolase isozymes in mouse sperm, two encoded by Aldoart1 and Aldoart2 retrogenes on different chromosomes and another by Aldoa-v2, a splice variant of Aldoa. Phylogenetic analyses and comparative genomics indicate that the retrogenes and splice variant have remained functional and have been under positive selection for millions of years. Their expression is restricted to the male germline and is tightly regulated at both transcriptional and translational levels. All three isozymes are present only in spermatids and sperm and have distinctive features that may be important for localization in the flagellum and/or altered metabolic regulation. Both ALDOART 1 and ALDOA-V2 have unusual N-teminal extensions not found in other aldolases. The N-terminal extension of ALDOA-V2 is highly conserved in mammals, suggesting a conserved function in sperm. We hypothesize that the N-terminal extensions are responsible for localizing components of the glycolytic pathway to the fibrous sheath and that this localization is required to provide sufficient ATP along the length of the flagellum to support sperm motility. (c) 2007 Elsevier Inc. All rights reserved.

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