Your search keyword '"Druzhinina, Marina"' showing total 3 results

1. Free and chromatin-associated mono-, di-, and trimethylation of histone H4-lysine 20 during development and cell cycle progression

Author

Karachentsev, Dmitry, Druzhinina, Marina, and Steward, Ruth

Subjects

*CHROMATIN, *CELL division, *AMINO acids, *CELL proliferation

Abstract

Abstract: Methylation of specific amino acids in histone tails is responsible for packaging DNA into condensed, repressed chromatin, and into open chromatin that is accessible to the transcription machinery. Monomethylation and trimethylation of histone H4-lysine 20 (H4-K20) control the formation of repressed chromatin. Using antibodies that specifically recognize the three methyl marks of histone H4-K20, we characterized their regulation during the cell cycle and throughout development. We find free mono- and trimethylated histone H4-K20 in unfertilized Drosophila eggs and in S2 tissue culture cells. Soluble mono-. di-, and trimethylated H4-K20 are also found in HeLa cells. These soluble modified histones may represent a pool of free histones that can rapidly be incorporated into chromatin. The three methyl marks are each regulated differentially during development and their detection on western blots does not overlap with their detection on chromosomes. Monomethylated H4-K20 is detected on condensed chromosomes throughout development, while di- and trimethylated H4-K20 are detected on metaphase chromosomes at specific stages. Our results suggest that the detection of methylated H4-K20 on chromosomes may reveal chromatin packaging rather than the distribution of the methyl marks. [Copyright &y& Elsevier]

Published

2007

2. spe-43 is required for sperm activation in C. elegans.

Author

Krauchunas, Amber R., Mendez, Ernesto, Ni, Julie Zhouli, Druzhinina, Marina, Mulia, Amanda, Parry, Jean, Gu, Sam Guoping, Stanfield, Gillian M., and Singson, Andrew

Subjects

*CAENORHABDITIS elegans, *SPERMATOZOA, *SPERMIOGENESIS in animals, *NUCLEOTIDE sequencing, *MEMBRANE proteins

Abstract

Successful fertilization requires that sperm are activated prior to contacting an oocyte. In C. elegans , this activation process, called spermiogenesis, transforms round immobile spermatids into motile, fertilization-competent spermatozoa. We describe the phenotypic and genetic characterization of spe-43 , a new component of the spe-8 pathway, which is required for spermiogenesis in hermaphrodites; spe-43 hermaphrodites are self-sterile, while spe-43 males show wild-type fertility. When exposed to Pronase to activate sperm in vitro , spe-43 spermatids form long rigid spikes radiating outward from the cell periphery instead of forming a motile pseudopod, indicating that spermiogenesis initiates but is not completed. Using a combination of recombinant and deletion mapping and whole genome sequencing, we identified F09E8.1 as spe-43 . SPE-43 is predicted to exist in two isoforms; one isoform appears to be a single-pass transmembrane protein while the other is predicted to be a secreted protein. SPE-43 can bind to other known sperm proteins, including SPE-4 and SPE-29, which are known to impact spermiogenesis. In summary, we have identified a membrane protein that is present in C. elegans sperm and is required for sperm activation via the hermaphrodite activation signal. [ABSTRACT FROM AUTHOR]

Published

2018

3. The sperm surface localization of the TRP-3/SPE-41 Ca2+-permeable channel depends on SPE-38 function in Caenorhabditis elegans

Author

Singaravelu, Gunasekaran, Chatterjee, Indrani, Rahimi, Sina, Druzhinina, Marina K., Kang, Lijun, Xu, X.Z. Shawn, and Singson, Andrew

Subjects

*CALCIUM channels, *SPERMATOZOA, *CAENORHABDITIS elegans, *GENETIC mutation, *FERTILIZATION (Biology), *OVUM

Abstract

Abstract: Despite undergoing normal development and acquiring normal morphology and motility, mutations in spe-38 or trp-3/spe-41 cause identical phenotypes in Caenorhabditis elegans—mutant sperm fail to fertilize oocytes despite direct contact. SPE-38 is a novel, four-pass transmembrane protein and TRP-3/SPE-41 is a Ca2+-permeable channel. Localization of both of these proteins is confined to the membranous organelles (MOs) in undifferentiated spermatids. In mature spermatozoa, SPE-38 is localized to the pseudopod and TRP-3/SPE-41 is localized to the whole plasma membrane. Here we show that the dynamic redistribution of TRP-3/SPE-41 from MOs to the plasma membrane is dependent on SPE-38. In spe-38 mutant spermatozoa, TRP-3/SPE-41 is trapped within the MOs and fails to reach the cell surface despite MO fusion with the plasma membrane. Split-ubiquitin yeast-two-hybrid analyses revealed that the cell surface localization of TRP-3/SPE-41 is likely regulated by SPE-38 through a direct protein–protein interaction mechanism. We have identified sequences that influence the physical interaction between SPE-38 and TRP-3/SPE-41, and show that these sequences in SPE-38 are required for fertility in transgenic animals. Despite the mislocalization of TRP-3/SPE-41 in spe-38 mutant spermatozoa, ionomycin or thapsigargin induced influx of Ca2+ remains unperturbed. This work reveals a new paradigm for the regulated surface localization of a Ca2+-permeable channel. [Copyright &y& Elsevier]

Published

2012