Upregulation of iNOS and phosphorylated eNOS in the implantation‐induced blastocysts of mice

Author:

Seki Misato1,Takeuchi Eisaku1,Fukui Emiko12,Matsumoto Hiromichi12ORCID

Affiliation:

1. Laboratory of Animal Breeding and Reproduction, Division of Animal Science, School of Agriculture Utsunomiya University Utsunomiya, Tochigi Japan

2. Center for Bioscience Research and Education Utsunomiya University Utsunomiya, Tochigi Japan

Abstract

AbstractPurposeThis study aimed to examine expressions of iNOS and phosphorylated eNOS (p‐eNOS) in implantation‐induced blastocysts. We also examined the upstream of p‐eNOS.MethodsTo address the protein expressions in implantation‐induced blastocysts, we performed immunohistochemical analysis using a delayed implantation mouse model. Immunostaining for iNOS, p‐eNOS, and p‐Akt was done. To address the relationship between p‐eNOS and p‐Akt, activated blastocysts were treated with an Akt inhibitor, MK‐2206.ResultsiNOS expression was at low levels in dormant blastocysts, whereas the expression was significantly increased in the activated blastocysts. Double staining of p‐eNOS and p‐Akt in individual blastocysts showed colocalization of p‐eNOS and p‐Akt of the trophectoderm. p‐eNOS and p‐Akt expressions were at low levels in dormant blastocysts, whereas both of them were significantly increased in the activated blastocysts. Both dormant and activated blastocysts showed significant positive correlations between p‐eNOS and p‐Akt. MK‐2206 treatment for activated blastocysts showed that blastocysts with lower p‐Akt had significantly lower p‐eNOS levels.ConclusionsiNOS and p‐eNOS, Ca2+ independent NOS, are upregulated by E2 in the blastocysts during implantation activation. Furthermore, p‐eNOS is upregulated in implantation‐induced blastocysts downstream of p‐Akt.

Funder

Japan Society for the Promotion of Science

Publisher

Wiley

Subject

Cell Biology,Reproductive Medicine

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