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KCIBackground : Exon deletions of Duchenne muscular dystrophy (DMD) gene account for most of the alterations found in DMD and Becker muscular dystrophy (BMD). This study was to evaluate the usefulness of dual priming oligonucleotide multiplex PCR (DPO PC...
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RISS 인기검색어
듀센형근이영양증 유전자의 결실 돌연변이 검출을 위한 Dual Priming Oligonucleotide 다중 PCR법의 평가 = Evaluation of Multiplex PCR Assay Using Dual Priming Oligonucleotide System for Detection Mutation in the Duchenne Muscular Dystrophy Gene
한글로보기https://www.riss.kr/link?id=A101631272
- 저자
- 발행기관
- 학술지명
- 권호사항
-
발행연도
2008
-
작성언어
Korean
- 주제어
-
등재정보
KCI등재,SCIE,SCOPUS
-
자료형태
학술저널
- 발행기관 URL
-
수록면
386-391(6쪽)
-
KCI 피인용횟수
1
- 제공처
-
0
상세조회 -
0
다운로드
부가정보
다국어 초록 (Multilingual Abstract)
Background : Exon deletions of Duchenne muscular dystrophy (DMD) gene account for most of the alterations found in DMD and Becker muscular dystrophy (BMD). This study was to evaluate the usefulness of dual priming oligonucleotide multiplex PCR (DPO PCR) in detection of exon deletions
of DMD gene.
Methods : Thirty-seven DMD or BMD patients who had known exon deletions detected by conventional multiplex PCR (conventional PCR) and nine control subjects were enrolled in this study. When a discrepancy was shown between the results of conventional PCR and DPO PCR, the multiplex
ligation-dependent probe amplification (MLPA) technique was performed as a confirmation test.
Results : The same deletions previously identified by conventional PCR in 32 out of 37 subjects were also detected by DPO PCR. For the five subjects (13.5%) showing discrepant results between the conventional PCR and DPO PCR, MLPA was performed and its results were found to correlate
better with those of DPO PCR. The discrepancies were due to false positive or false negative results of the conventional PCR.
Conclusions : DPO PCR shows a high agreement of results with the conventional PCR and is considered an adequate method to be used as a primary genetic test for the diagnosis of DMD. Because of an improved accuracy, especially for determining the boundaries of DMD gene deletions, DPO PCR can be very useful as a supplement to the conventional PCR. (Korean J Lab Med 2008;28:386-91)
of DMD gene.
Methods : Thirty-seven DMD or BMD patients who had known exon deletions detected by conventional multiplex PCR (conventional PCR) and nine control subjects were enrolled in this study. When a discrepancy was shown between the results of conventional PCR and DPO PCR, the multiplex
ligation-dependent probe amplification (MLPA) technique was performed as a confirmation test.
Results : The same deletions previously identified by conventional PCR in 32 out of 37 subjects were also detected by DPO PCR. For the five subjects (13.5%) showing discrepant results between the conventional PCR and DPO PCR, MLPA was performed and its results were found to correlate
better with those of DPO PCR. The discrepancies were due to false positive or false negative results of the conventional PCR.
Conclusions : DPO PCR shows a high agreement of results with the conventional PCR and is considered an adequate method to be used as a primary genetic test for the diagnosis of DMD. Because of an improved accuracy, especially for determining the boundaries of DMD gene deletions, DPO PCR can be very useful as a supplement to the conventional PCR. (Korean J Lab Med 2008;28:386-91)
Background : Exon deletions of Duchenne muscular dystrophy (DMD) gene account for most of the alterations found in DMD and Becker muscular dystrophy (BMD). This study was to evaluate the usefulness of dual priming oligonucleotide multiplex PCR (DPO PCR) in detection of exon deletions
of DMD gene.
Methods : Thirty-seven DMD or BMD patients who had known exon deletions detected by conventional multiplex PCR (conventional PCR) and nine control subjects were enrolled in this study. When a discrepancy was shown between the results of conventional PCR and DPO PCR, the multiplex
ligation-dependent probe amplification (MLPA) technique was performed as a confirmation test.
Results : The same deletions previously identified by conventional PCR in 32 out of 37 subjects were also detected by DPO PCR. For the five subjects (13.5%) showing discrepant results between the conventional PCR and DPO PCR, MLPA was performed and its results were found to correlate
better with those of DPO PCR. The discrepancies were due to false positive or false negative results of the conventional PCR.
Conclusions : DPO PCR shows a high agreement of results with the conventional PCR and is considered an adequate method to be used as a primary genetic test for the diagnosis of DMD. Because of an improved accuracy, especially for determining the boundaries of DMD gene deletions, DPO PCR can be very useful as a supplement to the conventional PCR. (Korean J Lab Med 2008;28:386-91)
참고문헌 (Reference)
1 Den Dunnen JT, "Topography of the Duchenne muscular dystrophy (DMD) gene: FIGE and cDNA analysis of 194 cases reveals 115 deletions and 13 duplications" 45 : 835-847, 1989
2 van Essen AJ, "The clinical and molecular genetic approach to Duchenne and Becker muscular dystrophy: an updated protocol" 34 : 805-812, 1997
3 Schouten JP, "Relative quantification of 40 nucleic acid sequences by multiplex ligation-dependent probe amplification" 30 : e57-, 2002
4 Den Dunnen JT, "Reconstruction of the 2.4 Mb human DMDgene by homologous YAC recombination" 1 : 19-28, 1992
5 Emery AE., "Population frequencies of inherited neuromuscular diseases--a world survey" 1 : 19-29, 1991
6 Chamberlain JS, "Multiplex PCR for the diagnosis of Duchenne muscular dystrophy in: PCR Protocols: A Guide to Methods and Applications" Academic Press 272-281, 1990
7 Ervasti JM, "Membrane organization of the dystrophin- glycoprotein complex" 66 : 1121-1131, 1991
8 Fujimura FK, "Genotyping errors with the polymerase chain reaction" 322 : 61-, 1990
9 Choi JR, "Genetic polymorphism analysis for the detection of Duchenne muscular dystrohpy carriers" 20 : 236-241, 2000
10 박수연, "Duchenne/Becker 근이영양증에서의 Dystrophin 유전자 분석" 대한소아신경학회 12 (12): 50-58, 2004
1 Den Dunnen JT, "Topography of the Duchenne muscular dystrophy (DMD) gene: FIGE and cDNA analysis of 194 cases reveals 115 deletions and 13 duplications" 45 : 835-847, 1989
2 van Essen AJ, "The clinical and molecular genetic approach to Duchenne and Becker muscular dystrophy: an updated protocol" 34 : 805-812, 1997
3 Schouten JP, "Relative quantification of 40 nucleic acid sequences by multiplex ligation-dependent probe amplification" 30 : e57-, 2002
4 Den Dunnen JT, "Reconstruction of the 2.4 Mb human DMDgene by homologous YAC recombination" 1 : 19-28, 1992
5 Emery AE., "Population frequencies of inherited neuromuscular diseases--a world survey" 1 : 19-29, 1991
6 Chamberlain JS, "Multiplex PCR for the diagnosis of Duchenne muscular dystrophy in: PCR Protocols: A Guide to Methods and Applications" Academic Press 272-281, 1990
7 Ervasti JM, "Membrane organization of the dystrophin- glycoprotein complex" 66 : 1121-1131, 1991
8 Fujimura FK, "Genotyping errors with the polymerase chain reaction" 322 : 61-, 1990
9 Choi JR, "Genetic polymorphism analysis for the detection of Duchenne muscular dystrohpy carriers" 20 : 236-241, 2000
10 박수연, "Duchenne/Becker 근이영양증에서의 Dystrophin 유전자 분석" 대한소아신경학회 12 (12): 50-58, 2004
11 Chun JY, "Dual priming oligonucleotide system for the multiplex detection of respiratory viruses and SNP genotyping of CYP2C19 gene" 35 : e40-, 2007
12 AH, Koenig M, "Detection of 98% of DMD/ BMD gene deletions by polymerase chain reaction" 86 : 45-48, 1990
13 Lai KK, "Detecting exon deletions and duplications of the DMD gene using Multiplex Ligationdependent Probe Amplification (MLPA)" 39 : 367-372, 2006
14 Koenig M, "Complete cloning of the Duchenne muscular dystrophy (DMD) cDNA and preliminary genomic organization of the DMD gene in normal and affected individuals" 50 : 509-517, 1987
15 Bergstrom DE, "Comparison of the base pairing properties of a series of nitroazole nucleobase analogs in the oligodeoxyribonucleotide sequence 5′-d(CGCXAATTYGCG)-3′" 25 : 1935-1942, 1997
16 Monaco AP, "An explanation for the phenotypic differences between patients bearing partial deletions of the DMD locus" 2 : 90-95, 1988
17 Ervasti JM, "A role for the dystrophin-glycoprotein complex as a transmembrane linker between laminin and actin" 122 : 809-823, 1993
18 Nobile C, "A refined restriction map of YAC clones spanning the entire human dystrophin gene" 5 : 566-571, 1994
19 Abbs S, "A convenient multiplex PCR system for the detection of dystrophin gene deletions: a comparative analysis with cDNA hybridisation shows mistypings by both methods" 28 : 304-311, 1991
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분석정보
인용정보 인용지수 설명보기
학술지 이력
| 연월일 | 이력구분 | 이력상세 | 등재구분 |
|---|---|---|---|
| 2023 | 평가예정 | 해외DB학술지평가 신청대상 (해외등재 학술지 평가) | |
| 2020-01-01 | 평가 | 등재학술지 유지 (해외등재 학술지 평가) | |
| 2012-05-21 | 학술지명변경 | 한글명 : The Korean Journal of Laboratory Medicine -> Annals of Laboratory Medicine외국어명 : The Korean Journal of Laboratory Medicine -> Annals of Laboratory Medicine | |
| 2011-01-01 | 평가 | 학술지 분리 (기타) | |
| 2010-06-29 | 학술지명변경 | 한글명 : 대한진단검사의학회지 -> The Korean Journal of Laboratory Medicine | |
| 2009-01-01 | 평가 | 등재학술지 유지 (등재유지) | |
| 2007-01-01 | 평가 | 등재학술지 유지 (등재유지) | |
| 2005-01-01 | 평가 | 등재학술지 유지 (등재유지) | |
| 2002-01-01 | 평가 | 등재학술지 선정 (등재후보2차) | |
| 1999-07-01 | 평가 | 등재후보학술지 선정 (신규평가) |  |
학술지 인용정보
| 기준연도 | WOS-KCI 통합IF(2년) | KCIF(2년) | KCIF(3년) |
|---|---|---|---|
| 2016 | 1.51 | 0.18 | 1.15 |
| KCIF(4년) | KCIF(5년) | 중심성지수(3년) | 즉시성지수 |
| 0.91 | 0.81 | 0.458 | 0.08 |
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