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centromere protein I OKDB#: 34
 Symbols: CENPI Species: human
 Synonyms: LRPR1, CENP-I, FSHPRH1  Locus: Xq22.1 in Homo sapiens


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General Comment Roberts et al. (1996) hypothesized that mutations in genes encoding components of the FSH signaling pathway might be responsible for cases of female or even male disorders of gonadal development. The rat gene called leucine-rich primary response gene 1 (LRPR1) is rapidly transcriptionally activated in response to FSH stimulation of rat testicular Sertoli cells, both in vitro and in vivo (Slegtenhorst-Eegdeman et al., 1995). Roberts et al. (1996) characterized a human transcript that probably encodes the ortholog of the rat protein. The gene encodes a 756-amino acid polypeptide with 72% identity to rat LRPR1 at the amino acid level. The gene maps to human chromosome Xq22 and therefore is a potential candidate for human X-linked disorders of gonadal development.

NCBI Summary: This gene encodes a centromere protein that is a component of the CENPA-NAC (nucleosome-associated) complex. This complex is critical for accurate chromosome alignment and segregation and it ensures proper mitotic progression. This protein regulates the recruitment of kinetochore-associated proteins that are required to generate the spindle checkpoint signal. The product of this gene is involved in the response of gonadal tissues to follicle-stimulating hormone. Mutations in this gene may be involved in human X-linked disorders of gonadal development and gametogenesis. Alternate splicing results in multiple transcript variants. A pseudogene of this gene is found on chromosome 13. [provided by RefSeq, Jan 2016]
General function
Comment
Cellular localization Cytoplasmic
Comment
Ovarian function
Comment
Expression regulated by
Comment In immature rat Sertoli cells LRPR1 represents a follicle stimulating hormone (FSH)-responsive gene; the function of the encoded protein is not yet known. LRPR1 mRNA expression is up-regulated very rapidly and specifically by FSH in rat testis. Similar studies in the ovary provided completely different results. LRPR1 mRNA in the postnatal ovary is present well before expression of FSHR mRNA can be first detected. In addition, incubation of ovaries of immature rats with FSH or dibutyryl cyclic AMP (dbcAMP) did not result in up-regulation of LRPR1 mRNA expression (Slegtenhorst-Eegdeman et al., 1998).
Ovarian localization
Comment
Follicle stages
Comment
Phenotypes POF (premature ovarian failure)
Mutations 1 mutations

Species: human
Mutation name:
type: naturally occurring
fertility: subfertile
Comment: Copy number variants on the X chromosome in women with primary ovarian insufficiency. Knauff EA et al. (2011) To investigate whether submicroscopic copy number variants (CNVs) on the X chromosome can be identified in women with primary ovarian insufficiency (POI), defined as spontaneous secondary amenorrhea before 40 years of age accompanied by follicle-stimulating hormone levels above 40 IU/L on at least two occasions. Analysis of intensity data of single nucleotide polymorphism (SNP) probes generated by genomewide Illumina 370k CNV BeadChips, followed by the validation of identified loci using a custom designed ultra-high-density comparative genomic hybridization array containing 48,325 probes evenly distributed over the X chromosome. Multicenter genetic cohort study in the Netherlands. 108 Dutch Caucasian women with POI, 97 of whom passed quality control, who had a normal karyogram and absent fragile X premutation, and 235 healthy Dutch Caucasian women as controls. None. Amount and locus of X chromosomal microdeletions or duplications. Intensity differences between SNP probes identify microdeletions and duplications. The initial analysis identified an overrepresentation of deletions in POI patients. Moreover, CNVs in two genes on the Xq21.3 locus (i.e., PCDH11X and TGIF2LX) were statistically significantly associated with the POI phenotype. Mean size of identified CNVs was 262 kb. However, in the validation study the identified putative Xq21.3 deletions samples did not show deviations in intensities in consecutive probes. X chromosomal submicroscopic CNVs do not play a major role in Caucasian POI patients. We provide guidelines on how submicroscopic cytogenetic POI research should be conducted. This gene showed copy number changes .//////////////////

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created: July 22, 1999, midnight by: Hsueh   email:
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last update: March 5, 2020, 3:58 p.m. by: hsueh    email:



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