PCR-RNA转录本分子杂交用于急性淋巴细胞白血病微小残留病的检测  

DETECTION OF MINIMAL RESIDUAL DISEASE IN ACUTE LYMPHOBLASTIC LEUKEMIA USING PCR MOLECULE HYBRIDIZATION OF RNA TRANSCRIPTS

在线阅读下载全文

作  者:梁欣荃[1] 费洪宝[1] 肖燕[1] 刘树茂[1] 杨爱德[1] 

机构地区:[1]同济医科大学附属协和医院儿科

出  处:《中华医学遗传学杂志》1998年第3期164-166,共3页Chinese Journal of Medical Genetics

基  金:国家自然科学基金

摘  要:目的为了快速、敏感地检测急性淋巴细胞白血病(急淋)微小残留病。方法以T细胞受体γ链基因重排为标志基因,将确诊时标本扩增后的PCR产物转录成放射标记的RNA探针,而不同病期标本的PCR产物转录成待测RNA,待测RNA与探针杂交后经RNaseA消化,之后再经聚丙烯酰胺凝胶电泳和放射自显影。结果急淋细胞系DNA对数稀释试验表明本方法的敏感度在10-5水平。1例急淋完全缓解期微小残留病也被成功地检测出来。而当探针和待测RNA并非来自同一个体时,交叉杂交的结果为阴性。Objective To detect acute lymphoblastic leukemia's (ALL's)minimal residual disease(MRD) rapidly and effectively. Methods In this assay, the gamma T cell receptor gene rearrangements serve as marker genes. The gene rearrangements are amplified from the diagnostic specimens using a consensus V segment primer and a consensus J segment primer to which the promoter T7 RNA polymerase has been appended. The PCR product from this amplification is transcribed into a radiolabeled RNA probe. The opposite DNA strand is transcribed into test RNA from the PCR product of different staged specimens. The test RNA is hybridized with the probe, and later the digestion with RNase A, Polyacrylamide gel electrophoresis and autoradiography are in progress. Results According to the mechanism, the perfectly matched RNA duplex can prevent the digestion of RNase A, and the presence of the leukemia cells in the test specimen can be determined. Logarithmical dilution experiments with DNA of a cell line from ALL have shown that this assay's sensitivity is at the 10 -5 level. Minimal residual disease was successfully detected in a case of ALL during its complete remission stage. But if the probe and test RNA are not from the same individual, the results of this kind of cross hybridization are negative. Conclusion The above results suggest that this assay can become an effective measure in the detection of ALL MRD clinically.

关 键 词:白血病 ALL 微小残留病 聚合酶链反应 

分 类 号:R733.710.4[医药卫生—肿瘤]

 

参考文献:

正在载入数据...

 

二级参考文献:

正在载入数据...

 

耦合文献:

正在载入数据...

 

引证文献:

正在载入数据...

 

二级引证文献:

正在载入数据...

 

同被引文献:

正在载入数据...

 

相关期刊文献:

正在载入数据...

相关的主题
相关的作者对象
相关的机构对象