PCR法检测粪便样本溶组织内阿米巴的初步研究

ObjectiveTo develop a PCR method forEntamoeba histolytica（E.histolytica) detection in fecal specimens, and to compare the performance of PCR to that of microscopy and ELISA.MethodsTwo pairs of self-designed primers and 2 pairs of primers from references based on small subunit ribosome RNA (SSU rRNA) fragment ofE. histolyticastandard strain were synthetized. DNA fromE. histolyticareference strain were amilified by the conventional PCR using the 4 pairs of primers. 221 stool samples from diarrhea patients were collected and detected forE. histolyticaby three methods:Entamoebatrophozoites and cysts detection by microscopy,E. histolytica-specific antigen detection using enzyme-linked immunosorbent assay (ELISA) kit (E. HISTOLYTICA II), amplification of SSU rRNA fragment ofE. histolyticaby PCR method. Positive rate of three methods were compared by chi-square test, andKappatest was applied to determine the concordance among the three methods.ResultsSpecific fragments ofE. histolyticawere amplified by the PCR method we developed in this study. Positive rates of PCR, microscopy and ELISA were 2.26%, 0.90% and 9.50%, respectively. The positive rates of the three methods were significantly different (χ²=23.34,P<0 .01). theKappavalue of PCR and microscopy was 0.216, and that of PCR and ELISA method was –0.134, both of which showed a weak consistency. PCR results showed best consistency with clinical diagnosis.ConclusionThe PCR method we established in this study has a better performance in accuracy than microscopy and ELISA have in laboratory diagnosis ofE. histolyticainfection.