Spam1-associated transmission ratio distortion in mice: Elucidating the mechanism
Spam1-associated transmission ratio distortion in mice: Elucidating the mechanism
AbstractBackgroundWhile transmission ratio distortion, TRD, (a deviation from Mendelian ratio) is extensive in humans and well-documented in mice, the underlying mechanisms are unknown. Our earlier studies on carriers of spontaneous mutations of mouse Sperm Adhesion Molecule 1 (Spam1) suggested that TRD results from biochemically different sperm, due to a lack of transcript sharing through the intercellular cytoplasmic bridges of spermatids. These bridges usually allow transcript sharing among genetically different spermatids which develop into biochemically and functionally equivalent sperm.ObjectivesThe goals of the study were to provide support for the lack of sharing (LOS) hypothesis, using transgene and null carriers of Spam1, and to determine the mechanism of Spam1-associated TRD.MethodsCarriers of Spam1-Hyal5 BAC transgenes were mated with wild-type female mice and the progeny analyzed for TRD by PCR genotyping. Sperm from transgene and Spam1 null carriers were analyzed using flow cytometry and immunocytochemistry to detect quantities of Spam1 and/or Hyal5. Transgene-bearing sperm with Spam1 overexpression were detected by fluorescence in situ hybridization. In wild-type animals, EM studies of in situ transcript hybridization of testis sections and Northern analysis of biochemically fractionated testicular RNA were performed to localize Spam1 transcript. Finally, AU-rich motifs identified in the 3' UTR of Spam1 RNA were assayed by UV cross-linking to determine their ability to interact with testicular RNA binding proteins.ResultsThe Tg8 line of transgene carriers had a significant (P < 0.001) TRD, due to reduced fertilizing ability of transgene-bearing sperm. These sperm retained large cytoplasmic droplets engorged with overexpressed Spam1 or Hyal5 protein. Caudal sperm from transgene carriers and caput sperm of null carriers showed a bimodal distribution of Spam1, indicating that the sperm in a male were biochemically different with respect to Spam1 quantities. Spam1 RNA was absent from the bridges, associated exclusively with the ER, and was shown to be anchored to the cytoskeleton. This compartmentalization of the transcript, mediated by cytoskeletal binding, occurs via protein interactions with 3' UTR AU-rich sequences that are likely involved in its stabilization.ConclusionWe provide strong support for the LOS hypothesis, and have elucidated the mechanism of Spam1-associated TRD.
- Thomas Jefferson University United States
- UNIVERSITY OF DELAWARE
- University of Delaware United States
- McGill University Canada
- ROYAL INSTITUTION FOR THE ADVANCEMENT OF LEARNING MCGILL UNIVERSITY Canada
Male, QH471-489, Genotype, Litter Size, Inheritance Patterns, Hyaluronoglucosaminidase, Mice, Transgenic, Mice, Animals, RNA, Messenger, Alleles, In Situ Hybridization, Fluorescence, Models, Genetic, Reproduction, Research, RNA-Binding Proteins, Gynecology and obstetrics, Seminiferous Tubules, Flow Cytometry, Spermatozoa, Mutation, RG1-991, Female, Cell Adhesion Molecules
Male, QH471-489, Genotype, Litter Size, Inheritance Patterns, Hyaluronoglucosaminidase, Mice, Transgenic, Mice, Animals, RNA, Messenger, Alleles, In Situ Hybridization, Fluorescence, Models, Genetic, Reproduction, Research, RNA-Binding Proteins, Gynecology and obstetrics, Seminiferous Tubules, Flow Cytometry, Spermatozoa, Mutation, RG1-991, Female, Cell Adhesion Molecules
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