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KISSFagile X syndrome is the most common cause of inherited mental retardation. The diagnosis of fragile X syndrome was originally based on the expression of a folate-sensitive fragile site at X chromosome(Xq27.3) in cell culture under conditions of folat...
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RISS 인기검색어
한국인 취약 X증후군 환자 및 보인자의 분자유전학적 양상과 진단 = Molecular Genetic Analysis of Korean Patients with Fragile X Syndrome
한글로보기https://www.riss.kr/link?id=A3360028
- 저자
- 발행기관
- 학술지명
- 권호사항
-
발행연도
1996
-
작성언어
-
- 주제어
-
KDC
500
-
등재정보
KCI등재,SCOPUS,ESCI
-
자료형태
학술저널
- 발행기관 URL
-
수록면
854-864(11쪽)
- 제공처
-
0
상세조회 -
0
다운로드
부가정보
다국어 초록 (Multilingual Abstract)
Fagile X syndrome is the most common cause of inherited mental retardation. The diagnosis of fragile X syndrome was originally based on the expression of a folate-sensitive fragile site at X chromosome(Xq27.3) in cell culture under conditions of folate deprivation. The cytogenetic study test has limitations, especially in testing for carrier status, and it exhibites a high degree of variability between individuals and laboratories. In 1991, the fragile X gene(FMR-1) was characterized and the nature of the fragile X mutation has been elucidated. At present in developed countries, DNA testing has been utilized in the diagnosis of fragile X syndrome and its carriers. This study was undertaken to analysis the FMR-1 gene in Korean patients with fragile X syndrome and tis carriers and to establish the methodology for molecular genetic diagnosis of fragile X syndrome and its carrier. Three male patients with fragile X syndrome previously diagnosed by cytogenetic analysis and their family members, as well as 16 persons proven cytogenetically normal were analysed by direct genomic Southern blot anlysis and polymerase chain reaction (PCR) for the status of FMR-1 gene. Southern blot analysis consisted of double DNA digestion with Eag I and EcoRI and the hybridization whth StB 12.3 probe. Two kinds of PCR methods were used. The one method involved the addition of radio-active dNTP in PCR reaction, and the other involved Southern trnsfer of amplified PCR products and the hybridization analysis with synthetic oligonucletide probe. In normal female and male, firect genomic Southern blot analysis revealed the patterns as follows: 2.8 kb band in normla male, and 2.8kb band in normal female. And the patients(male) with fragile X syndrome showed the band sized more than 5.8 kb with 5.2 band. The father of a patient with fragile X syndrome showed the normal pattern. PCR analysis of the cytogeneticaly normal males and females revleaed the normal patterns, namely the bands of sizes expected from the primers used. However, either PCR method failed to reveal full mutation alleles in patients with fragile X syndrome. And premutation alleles could be detected in two mothers of patients by PCR method. The father of a patient with fragile X syndrome showed the normal pattern by either PCR method. Thses data suggest that Southern blot analysis can be used in the accurate diagnosis of fragile X syndrome and its carrier and that PCR method can be utilized to exclude the diagnosis of fragile X syndrome in unaffected males.
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