赣南地区客家人重型地中海贫血基因突变类型分析及防治的研究

目的:探讨赣南地区客家人重型地中海贫血基因突变类型及其比例,为本地区地中海贫血的防治、指导遗传咨询及流行病学研究提供一定的参考数据。方法:选择2009年1月-2019年1月赣南医学院第一附属医院收治的客家人重型地中海贫血患者81例,采用跨越断裂点PCR(Gap-PCR)法检测缺失型α-地中海贫血,采用PCR-反向点杂交(PCR-RDB)法检测α-地中海贫血点突变和β-地中海贫血点突变,对我院81例客家人重型地中海贫血患者进行地中海贫血基因检测分析,计算基因突变频率。结果:在81例客家人重型地中海贫血患者中,共检出4种β-地中海贫血(纯合子)基因型,依次是CD41-42(-TTCT)(19例)、β-IVS-II-654(C→T)(9例)、-28M(A→G)(1例)、CD17(A→T)(1例);12种β-地中海贫血(杂合子)基因型,依次是CD41-42(-TTCT)/β-IVS-II-654(C→T)(15例,29.41%),β-IVS-II-654(C→T)/β-28M(A→G)(13例,25.49%);CD41-42(-TTCT)/β-28M(A→G)(9例,17.65%);β-IVS-II-654(C→T)/CD27/28(+C)(3例,5.88%);CD41-42(-TTCT)/CD27/28(+C)(3例,5.88%);β-28M(A→G)/CD17(A→T)(2例,3.92%);CD41-42(-TTCT)/CD17(A→T)、CD41-42(-TTCT)/Βe、β-IVS-II-654(C→T)/β-29、βCD17(A→T)/CD71-72(+a)、βCD71-72/β-28M(A→G)、β-28M(A→G)/β-IVS-II-654(C→T)(各1例,各占1.96%)。β纯合地中海贫血合并α地中海贫血基因3例,β杂合地中海贫血合并α地中海贫血基因5例。结论:江西赣南地区客家人重型β-地中海贫血发病率较高,其基因突变类型分布情况如下:β-地中海贫血(纯合子)以CD41-42(-TTCT)基因型为主;β-地中海贫血(杂合子)以CD41-42(-TTCT)/β-IVS-II-654(C→T)及β-IVS-II-654(C→T)/β-28M(A→G)两种基因型为主;β复合α地中海贫血以CD41-42(-TTCT)基因为主。

PBL与CBL教学法在医学微生物学课程中应用及效果评价

目的探讨以案例为基础的教学方法(CBL)和以问题为导向的教学方法(PBL)在医学微生物学教学中的应用效果。方法随机抽取本校2014级临床医学专业本科1~6班的同学作为调查对象,采用问卷调查、统计学方法和课程考核的方式进行分析。结果显示与CBL教学法相比,PBL有13个项目相对于CBL具有优势(P<0.05);运用传统讲授法结合PBL法的学生成绩最高,显著高于运用其他两种方法的学生成绩,其次是运用传统讲授法结合CBL法的成绩显著高于单纯传统讲授法。结论 PBL教学法更容易实现理论和实践相结合,提高学生学习的主动性,并对提高语言表达能力、人际沟通能力和团队合作意识等综合素质有明显帮助,其教学效果明显优于CBL教学法。由此,提出在医学微生物学教学过程中以PBL为主,CBL为辅,两者互相补充,综合运用,才能最大限度地提高教学质量。

An Evaluation of the Infection Status and Source of Subgroup J Avian Leukosis Virus in Cloned Free-Range Layers

In recent years, subgroup J avian leukosis virus （ALV-J） has been found to frequently infect layers in China. This virus is responsible for economic losses due to both mortality and decreased performance in chickens. In this study, 45-d-old cloned flee-range layers were suspected to be infected with ALV and other immunosuppressive diseases because their feathers were unkempt and their growth rate was impaired. To estimate the infection status and determine the source of ALV-J in the flock, 30 cloacal swabs were randomly collected to measure the p27 antigen level by enzyme-linked immunosorbent assay （ELISA）. Among the birds that were tested, 87% （26/30） were positive. In addition, 6 anticoagulant blood samples were aseptically collected at random from the flock when the layers were 60 d old. These samples were centrifuged to obtain the leukocytes, which were then used to inoculate chicken embryo fibroblast （CEF） cells for the identification of ALV-J by indirect immunofluorescence （IFA）. Of the samples tested, 100% （6/6） were positive. The flock＇s production performance was also investigated, and 10 layers were necropsied to evaluate pathological changes at 115 d of age. The flock never laid eggs even though they reached the age of the first laying （110 d）. Furthermore, there were pathological changes present, including atrophy of the thymus and bursa of Fabricius, undeveloped ovaries, glandular stomach haemorrhage, and hepatosplenomegaly. Paraffin-embedded sections of intumescent liver and spleen were prepared for antigen localisation using IFA. Positive signals were prevalent in paraffin-embedded sections of the intumescent liver and spleen. Furthermore, provirus DNA was extracted from 4 cloned flee-range layers, and 2 patemal parents （HR native cocks）, and the gp85 gene of ALV-J was amplified by PCR to analyse the genetic variation. The results of the autogenous variation analysis showed that the 6 strains were 98.5-99.7% homologous. This study indicated that there was persistent infection with ALV-J by dynamic inspection, which seriously reduced the production performance of the flock. In addition, the genetic variation analysis showed that ALV-J in the flock was more likely to have originated from the paternal parent, the HR native cock.