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Evaluation of clinical application of gap-PCR as a routine method for alpha-thalassemia carrier detection.

作者信息

Zhou Yu-Qiu, Xiao Ge-Fei, Li Li-Yan, Li Wen-Dian, Liu Zhong-Ying, Zhu Lan-Fang, Mo Qiu-Hua, Qu Xin-Jun, Xu Xiang-Min

机构信息

Women and Children's Healthcare Hospital of Zhuhai City, Zhuhai 519001, China.

出版信息

Di Yi Jun Yi Da Xue Xue Bao. 2002 May;22(5):434-6.

Abstract

OBJECTIVE

To evaluate the feasibility of using gap-PCR for routine screening of alpha-thalassemia in clinical laboratory.

METHODS

A total of 382 clinical blood samples randomly collected from the population of Zhuhai city were screened for alpha-thalassemia determinants with hematological and gap-PCR method respectively in a double-blind manner. Parallel analysis with Southern blotting was performed to verify the genotyping results by PCR.

RESULTS

Of the 382 samples tested, 3 common alpha-thalassemia genes with genotypes of --(SEA)/alpha alpha, -alpha(3.7)/alpha alpha and -alpha(4.2)/alpha alpha were detected in 21 (5.50%), 7 (1.83%) and 3 (0.79%) cases respectively by gap-PCR, including 7 cases with normal phenotype and 3 case of iron-deficiency anemia. The overall incidence of alpha-thalassemia was 8.12% in the population of Zhuhai city, as determined by gap-PCR, in total agreement with the results by Southern blotting. Only 21 of the 31 alpha-thalassemia cases were identified by hematological analysis (besides 2 cases with alpha-thalassemia phenotype undetermined), which had a false-negative rate of 32.3%. Seven silent alpha-thalassemia and 3 mild alpha-thalassemia cases failed to be detected by hematological analysis, resulting in a rate of 2.62% for failure of detection.

CONCLUSION

Gap-PCR method is specific and feasible as a better alternative for alpha-thalassemia screening, especially advantageous in detecting silent carriers in comparison with hematological method.

摘要

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