RAPID METHOD FOR DISTINGUISHING CLONAL FROM POLYCLONAL B-CELL POPULATIONS IN SURGICAL BIOPSY SPECIMENS

被引：206

作者：

MCCARTHY, KP ^{[1
]}

SLOANE, JP ^{[1
]}

WIEDEMANN, LM ^{[1
]}

机构：

[1] ROYAL MARSDEN HOSP,DEPT HISTOPATHOL,SUTTON SM2 5PT,SURREY,ENGLAND

来源：

JOURNAL OF CLINICAL PATHOLOGY | 1990年 / 43卷 / 05期

关键词：

D O I：

10.1136/jcp.43.5.429

中图分类号：

R36 [病理学];

学科分类号：

100104 ;

摘要：

The polymerase chain reaction (PCR) was used to detect clonal rearrangements of the immunological heavy chain gene in frozen samples of human lymphoid tissue. DNA sequences in rearranged genes were amplified using oligomeric primers predicted from conserved sequences in the variable (V(H)) and joining (J(H)) regions. On polyacrylamide gel electrophoresis, polyclonal B cell proliferations showed a 'smear', probably due to the variable lengths of the diversity (D(H)) region genes and the N regions separating the V(H) and D(H) and J(H) regions. In contrast, DNA from B cell lymphomas showed a clear single band in eight out of 10 cases. PCR undertaken on germ line DNA from nonlymphoid tumours showed no detectable bands or smears. The method can be completed within one day of biopsy, compared with several days in the case of conventional DNA blot analysis. Furthermore, it is cheaper, simpler, avoids the need for radioactive materials and requires very small amounts of DNA (about 1 μg).

引用

页码：429 / 432

页数：4

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