GENOMIC CLONING AND LOCALIZATION BY FISH AND LINKAGE ANALYSIS OF THE HUMAN GENE ENCODING THE PRIMARY SUBUNIT NMDAR1 (GRIN1) OF THE NMDA RECEPTOR-CHANNEL

被引：8

作者：

BRETT, PM

LEBOURDELLES, B

SEE, CG

WHITING, PJ

ATTWOOD, J

WOODWARD, K

ROBERTSON, MM

KALSI, G

POVEY, S

GURLING, HMD

机构：

[1] MERCK SHARP & DOHME LTD, RES LABS, HARLOW CM20 2QR, ESSEX, ENGLAND

[2] UCL, GALTON LAB, MRC, HUMAN BIOCHEM GENET UNIT, LONDON NW1 2HE, ENGLAND

[3] UCL, GALTON LAB, DEPT GENET & BIOMETRY, LONDON NW1 2HE, ENGLAND

来源：

ANNALS OF HUMAN GENETICS | 1994年 / 58卷

关键词：

D O I：

10.1111/j.1469-1809.1994.tb01879.x

中图分类号：

Q3 [遗传学];

学科分类号：

071007 ; 090102 ;

摘要：

A cDNA clone of the NMDAR1 (isoform E) has been used to screen both lambda and cosmid genomic libraries. A genomic phage clone was identified and sequenced and was found to contain some of the 3' coding regions of the GRIN1 gene. This clone was used to localize the gene using fluorescent in situ hybridization (FISH) to normal chromosomes, and also to a lymphoblastoid cell line containing a translocation involving chromosomes 9 and 15. FISH localized the gene to chromosome 9q34.3. The clone was used to screen a panel of genomic DNAs cut with 20 restriction enzymes. A VNTR sequence 5' to the gene, which was polymorphic for a number of restriction enzymes, was detected. A PvuII fragment of the genomic clone was found to detect the VNTR on Southern hybridization. The polymorphic VNTR marker was mapped against chromosome 9q34 markers using linkage analysis in the CEPH families. The GRIN1 gene was linked to D9S7 with a maximum lod score of 20.09 at zero recombination fraction in males and 0.03% recombination in females.

引用

页码：95 / 100

页数：6

共 23 条

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