| First Author | Furuichi T | Year | 2019 |
| Journal | Mamm Genome | Volume | 30 |
| Issue | 11-12 | Pages | 329-338 |
| PubMed ID | 31776724 | Mgi Jnum | J:281887 |
| Mgi Id | MGI:6379968 | Doi | 10.1007/s00335-019-09822-3 |
| Citation | Furuichi T, et al. (2019) Crim1(C140S) mutant mice reveal the importance of cysteine 140 in the internal region 1 of CRIM1 for its physiological functions. Mamm Genome 30(11-12):329-338 |
| abstractText | Cysteine-rich transmembrane bone morphogenetic protein regulator 1 (CRIM1) is a type I transmembrane protein involved in the organogenesis of many tissues via its interactions with growth factors including BMP, TGF-beta, and VEGF. In this study, we used whole-exome sequencing and linkage analysis to identify a novel Crim1 mutant allele generated by ENU mutagenesis in mice. This allele is a missense mutation that causes a cysteine-to-serine substitution at position 140, and is referred to as Crim1(C140S). In addition to the previously reported phenotypes in Crim1 mutants, Crim1(C140S) homozygous mice exhibited several novel phenotypes, including dwarfism, enlarged seminal vesicles, and rectal prolapse. In vitro analyses showed that Crim1(C140S) mutation affected the formation of CRIM1 complexes and decreased the amount of the overexpressed CRIM1 proteins in the cell culture supernatants. Cys140 is located in the internal region 1 (IR1) of the N-terminal extracellular region of CRIM1 and resides outside any identified functional domains. Inference of the domain architecture suggested that the Crim1(C140S) mutation disturbs an intramolecular disulfide bond in IR1, leading to the protein instability and the functional defects of CRIM1. Crim1(C140S) highlights the functional importance of the IR1, and Crim1(C140S) mice should serve as a valuable model for investigating the functions of CRIM1 that are unidentified as yet. |
