聚合酶链反应检测铜绿假单胞菌感染性角膜溃疡的实验研究及临床应用

目的：探索聚合酶链反应（PCR）技术对铜绿假单胞菌感染性角膜溃疡快速诊断的可行性。优越性及其在临床应用中的价值。方法：建立PCR检测标准铜绿假单胞菌方法，对兔铜绿假单胞菌感染性角膜溃疡模型研究并应用于临床，并与细菌培养做比较。结果：铜绿假单胞菌扩增出一条长504bp的阳性条带，其他常见细菌，人和兔正常角膜组织均为阴性，动物模型PCR敏感性为93.8%。特异性为100.0%；细菌培养敏感性为68.7%。特异性为93.7%。临床标本PCR阳性率为66.7%；细菌培养阳性率为38.1%。结论：PCR技术对快速检测实验室和临床标本中的铜绿假单胞菌具有重要的应用价值。     

PCR-RSSO基础上HLA-Ⅰ、Ⅱ基因分型的研究

目的通过对PCR-DNA技术的分析,探讨人类白细胞抗原(HLA)基因分型方法。方法采用PCR反向序列特异性寡核苷酸(polymerase chain reaction-reverse sequence specific oligonucleotide,PCR-RSSO)杂交技术,建立改良半量扩增体系全自动HLA-I、Ⅱ等位基因分型方法,进行了635份血液标本HLA-A、B、C、DR、DQ等位基因分型,其中166份DNA同时采用序列特异性引物技术(PCR-SSP)和手工全量扩增体系PCR-RSSO技术。对全自动半量PCR-RSSO、PCR-SSP、手工PCR-RSSO 3种方法做两两比较。结果全自动半量PCR-RSSO的分型成功率为98.4%(3 124/3 175),PCR-SSP为98.8%(656/664),手工PCR-RSSO为88.3%(733/830)。经χ2检验,全自动半量PCR-RSSO与PCR-SSP的分型成功率无统计学差异,与手工PCR-RSSO有显著差异(P<0.05)。结论PCR-RSSO可识别HLA-Ⅰ,Ⅱ共706个等位基因,覆盖WHO命名委员会2000年公布的936个等位基因的75.43%;对706个HLA等位基因的分型均为中~高分辨率,有分辨纯合子等位基因的能力;易长期保存书面的实验原始资料,即杂交条;具有成本低、劳动强度低、省时和DNA消耗量少等优点。PCR-RSSO适合于造血干细胞移植和建立造血干细胞及脐带血干细胞库的组织配型。     

小干扰RNA干扰大鼠神经元Nogo受体mRNA表达的实验研究

目的观察大鼠Nogo受体(NgR)特异性小干扰RNA(small interfering RNA,siRNA)在原代神经元干扰其mRNA表达的效果。方法体外培养大鼠原代皮层和海马细胞,应用阳离子脂质体转染试剂转染4对化学合成的大鼠NgR特异性siRNA,72h后提取细胞总RNA,实时荧光定量RT-PCR检测NgR mRNA表达情况。结果4对siRNA均能够下调靶基因NgR的mRNA表达水平,siNgR199、siNgR562、siNgR772和siNgR964等干扰后,NgR mRNA的表达分别为对照siRNA干扰组的6.5%、62.4%、15.2%和6.86%,与对照siRNA干扰组比较有统计学意义(P<0.05)。结论化学合成的NgR特异性siRNA能够有效的干扰大鼠原代皮层和海马细胞内NgR基因mRNA的表达水平。     

Aspergillus Iris Granuloma: A Case Report with Review of Literature

We report the case of a 25-year-old male patient who presented with complaints of redness, photophobia, and decreased vision in the right eye of a week's duration. Slit-lamp biomicroscopic examination revealed a cream-colored, irregular elevated inferior iris mass, extending on to the anterior lens surface. Differential diagnoses of a fungal granuloma, a medulloepithelioma, and an amelanotic melanoma were considered. An excisional biopsy of the mass was performed through a superior clear corneal incision. Polymerase chain reaction analysis of the aqueous humor showed a positive pan fungal genome. Histopathology of the biopsied mass showed a giant cell granuloma with surrounding numerous branching, septate hyphae. Culture growth revealed Aspergillus fumigatus We report this case because of the rarity of Aspergillus iris granuloma as a primary presentation of endogenous Aspergillosis and review the relevant literature. Absence of a significant systemic history compounded the diagnostic dilemma in our patient. Definitive differentiation of this rare entity from a foreign body, amelanotic melanoma, and other inflammatory conditions such as sarcoidosis and tuberculosis, may be possible only on microbiological and histo-pathological evaluation.     

D16S539等5个短串联重复序列基因座遗传多态性分析

目的　探讨河南汉族群体 D16S53 9、D7S82 0、D13 S3 17、D8S1179和 D2 1S11等 5个基因座基因频率 ,获得群体遗传学数据。方法　随机抽取 2 0 9名河南汉族群体无血缘关系个体的静脉血 ,柠檬酸抗凝剂抗凝 ,酚 -氯仿法提取 DNA ,应用 PCR技术扩增上述 5个 STR基因座 ,聚丙烯酰胺凝胶垂直板电泳分型。结果　 2 0 9名个体中 D16S53 9、D7S82 0、D13 S3 17、D8S1179和 D2 1S11等 5个基因座分别检出 7、8、8、10、15个等位基因 ,基因型分布符合 Hardy-Weinberg平衡。 5个基因座的杂合度分别为 0 .790 7、0 .80 56、0 .7914、0 .82 3 9、0 .80 46,多态信息含量分别为 0 .7712、0 .780 1、0 .7694、0 .80 0 9、0 .7816,个人识别能力在 0 .9416、0 .93 67、0 .9511、0 .9546、0 .93 0 8,非父排除概率分别为 0 .610 6、0 .6179、0 .614 5、0 .70 2 2、0 .6712。结论　 5个 STR基因座具有高度多态性遗传标记特征 ,在群体遗传学研究和法医学应用中具有较高的价值     

乙型肝炎患者血清中分泌型IgA水平与HBV DNA含量的关系

湖北省鹤峰县人民医院检验科,鹤峰 445800目的 研究乙型肝炎患者血清中分泌型IgA(SIgA)水平与乙型肝炎病毒(HBV)DNA含量的关系,为临床提供一个新的评价HBV复制状态及肝细胞损伤的指标。方法 100份经ELISA检测并确诊为乙型肝炎的患者血清用荧光定量PCR检测HBV DNA的拷贝数,用ELISA并经酶标仪定量其SIgA的量。结果 SIgA的含量与HBVDNA的拷贝数的对数呈正相关(r=0.69,P<0.01),在HBsAg( )/HBeAg( )/HBcAb( )组和HBsAg( )/HBeAb( )/HBcAb( )组中SIgA含量差异无显著性意义(P>0.05),而HBV DNA拷贝数前者明显高于后者(P<0.01)。结论 乙型肝炎患者血清SIgA的含量在评价HBV的传染性及肝细胞损伤程度方面比乙型肝炎血清学标志物(HBV-M)更灵敏、准确。     

Expression of myosin heavy chain isoforms in Duchenne muscular dystrophy patients and carriers

The expression of MHC isoforms in the skeletal muscles of nine patients with Duchenne muscular dystrophy (DMD) (from 2.5 to 15 yr of age) and three DMD carriers was studied using different specific anti-MHC MAbs. We also analyzed muscle fiber size and fiber reactivity with acridine orange and/or with a surface antigen marker. One-quarter of all fibers of DMD patients, or less with age, were of normal size and contained only adult slow MHC. Half of the muscle fibers contained adult and developmental MHCs. Only half of these fibers were representative of an active regenerative process. MHC co-expression also altered the proportion of normal fast or slow fibers. Adult fast MHCs were expressed as unique MHC only in small and very small fibers in the oldest DMD patients. In DMD carrier muscles, the greatest alterations in MHC expression were observed in patients with the most reduced dystrophin expression. However, MHC changes in dystrophin-positive fibers were similar to those observed in dystrophin-free fibers. In conclusion, disruptions or delays in the switching of all genes coding for adult fast and slow MHC and developmental MHC coincided with dystrophin deletion and with perturbations in its expression.