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991.
A polymerase chain reaction (PCR)-based test was developed for the detection of mecA in staphylococci. To facilitate this process, a rapid cell lysis procedure was established for the release of DNA from staphylococcal strains. Primers based on the DNA sequence of the mecA gene from Staphylococcus aureus were used in PCRs to screen for the presence of this gene in a total of 98 staphylococcal isolates. Fifty-one isolates were mecA positive (17 S. aureus strains and 34 coagulase-negative staphylococci including S. epidermidis, S. haemolyticus, and S. simulans). Results obtained with PCRs were generally consistent with those of standard microbiological assays. PCRs designed to detect the femA gene (factor essential for methicillin resistance) revealed the presence of the gene in all S. aureus strains examined regardless of the susceptibility profiles of the strains to methicillin. In contrast, femA could not be detected in coagulase-negative staphylococci by PCR with the same primers. Low-stringency hybridization suggested the presence of a gene structurally related to femA in S. epidermidis and other coagulase-negative staphylococci examined.  相似文献   
992.
To assess the immune recognition of DNA in systemic lupus erythematosus, the antigenic specificity of monoclonal anti-DNA antibodies from autoimmune MRL-lpr/lpr mice was investigated Determinant specificity was assessed by ELISA in terms of binding to a panel of ssDNA antigens including calf thymus, human placenta, Escherichia coli, Clostridium perfringens, Micrococcus lysodeikticus, salmon testes, chicken blood and murine DNA. Among the monoclonal antibodies, a variety of binding patterns was observed, although for all antibodies tested murine DNA was among the most reactive antigens. Binding to other DNAs varied markedly, with some antibodies showing only low reactivity to certain antigens in the test panel. Similar results were obtained with sera of individual MRL-lpr/lpr mice. These results suggest that anti-DNA antibodies bind specific antigenic determinants variably expressed by DNAs of various species. Furthermore, the preferential binding to mouse DNA by some MRL-lpr/lpr antibodies may suggest a role of self-DNA in the in vivo selection of anti-DNA antibodies for expression.  相似文献   
993.
目的:评价医用生物蛋白胶(BFG)联合大网膜包肾(ORP)对门静脉高压症患者断流术后近期和远期疗效的影响。方法:将我院3年内(2003年11月~2006年5月)收治的118例门静脉高压症接受选择性贲门周围血管离断术(sPCDV)患者分成两组,即应用BFG联合ORP组(A组,n=72)和对照组(B组,n=46),比较两组手术后近期(一月)脾窝渗液、发热和远期上消化道再出血、肝性脑病和胃病等并发症的发生率。结果:A组手术近期脾窝渗液和发热率明显低于B组(P<0.05);A组和B组随访期间上消化道再出血率分别为1.3%和10.8%(P<0.05)、门静脉高压性胃病发生率分别为30.6%和65.2%(P<0.05);A组肝性脑病发生率与B组无明显差异(P>0.05)。结论:BFG联合ORP可有效降低选择性断流术后近期和远期并发症的发生,提高门静脉高压症患者断流术的疗效。  相似文献   
994.
为了研究NMDA受体活性对Aβ引发的海马神经元突触蛋白表达变化的影响,本文运用免疫细胞化学方法检测不同浓度NMDA受体激动剂以及拮抗剂对Aβ诱导的海马神经元突触蛋白变化的影响。结果显示:NMDA可浓度依赖性地缓解Aβ25-35引起的突触蛋白synaptophysin与PSD-95的减少。抑制突触内NMDA受体,NMDA缓解Aβ减少突触蛋白的作用减弱;抑制突触外NMDA受体,对抗Aβ的作用无显著变化。本研究结果提示NMDA受体活性改变影响Aβ诱导的突触蛋白减少,突触内NMDA受体激活可对抗Aβ的毒性作用。突触内NMDA受体活性减弱可能在谷氨酸兴奋毒性中发挥作用。  相似文献   
995.
996.
采用聚合酶链反应(PCR)技术,对42例肝活切组织石蜡切片中乙型肝炎病毒(HBV)DNA进行检测,并与乙肝表面抗原(HBsAg)的免疫组织化学及血清学检测进行比较,HBV-PCR阳性率为73.8%,高于组织及血清HBsAg阳性率(分别为59.5%和50.0%)。3例病理形态呈肝炎改变,而血清HBsAg(─)的肝组织中有2例检出HBV-DNA,提示PCR的高度敏感性和准确性。83.3%的门脉性肝硬变和87.5%的肝细胞癌组织中HBV-PCR呈阳性,进一步证实了上述两病与HBV的关系密切。我们还发现肝细胞淤胆患者HBV感染率较高,HBV-DNA及组织HBsAg阳性比例各为6/9和4/8。  相似文献   
997.
Mg^2+对离体灌流内皮素的大鼠心脏功能的影响   总被引:1,自引:0,他引:1  
本实验在离体大鼠心脏灌流模型上,观察到10~(-9)mol/L内皮素灌流引起心肌挛缩,心功能降低,冠脉灌流量减少,以及心肌Ca~(2 )聚积,Mg~(2 )丧失等表现。灌流液含低镁(0.12mmol/L)时内皮素对心脏的上述作用显著增强,而在含高镁(4.8mmol/L)时明显减弱。Mg~(2 )影响内皮素对心脏作用的机制可能与其抑制心肌Ca~(2 )内流有关。实验结果提示避免缺镁,适当补充Mg~(2 )对于防治伴有循环内皮素水平增加的疾病或病理过程中的心脏损伤可能具有临床意义。  相似文献   
998.
目的:了解肺炎克雷伯杆菌与膀胱上皮细胞的相互关系,观察肺炎克雷伯杆菌在人膀胱上皮细胞抹T24中生存的动态变化。方法:采用肺炎克雷伯杆菌临床分离抹03138侵袭T24细胞,并用庆大霉素杀死细胞外的细菌,分别于细菌进入细胞后的4、24、48及72h裂解细胞,释放出细胞内的活细菌,用平板菌落计数法计数胞内活菌数。结果:T24细胞内的肺炎克雷伯杆菌03138抹在实验48h内有一定生长,试验72h细胞内活菌数量明显减少。加入细胞因子(TNF-αd和INF-γ)可以促进上皮细胞清除胞内细菌。结论:膀胱上皮细胞清除进入细胞内的肺炎克雷伯杆菌,可能是泌尿道天然免疫的一种防御机制,而细胞因子可以调控上皮细胞的抗菌作用。  相似文献   
999.
Our purpose in this work was to assess the reliability of the calibration coefficient for magnetic resonance water proton chemical shift temperature mapping. Over a six month period, the calibration coefficient was measured 15 times in several different phantoms. A highly linear relationship between water proton chemical shift and temperature change was found. The average temperature calibration coefficient determined from all studies was 0.009+/-0.001 ppm/degrees C. Four of the 15 studies were conducted on the same day using the same phantom. The average temperature calibration coefficient of these four studies was 0.0096+/-0.0001 ppm/degrees C.  相似文献   
1000.
Vascular adhesion protein-1 (VAP-1) is an adhesion molecule controlling lymphocyte recirculation through high endothelial venules of the lymph nodes. It has also been shown to be induced and to mediate lymphocyte adhesion at sites of inflammation. We studied the expression of VAP-1 and two other inducible adhesion molecules ICAM-1 and VCAM-1 in our experimental model of rat liver allograft rejection and, in addition, the effect of concomitant rat cytomegalovirus (RCMV) infection on this expression. Expression of VAP-1, ICAM-1, and VCAM-1 was studied in rat liver allografts with or without RCMV infection, isografts, and normal rat liver. Immunoperoxidase technique and monoclonal antibodies including a novel anti-VAP-1 reagent were used. VAP-1 expression was induced by acute rejection in sinusoids, hepatocytes, and also in bile ducts, when compared to the isografts or normal liver, where only blood vessels were consistently positive. Sinusoidal and hepatocyte expression of VAP-1 was prolonged by the presence of RCMV. ICAM-1 and VCAM-1 expression was also induced by acute rejection. However, RCMV increased sinusoidal VCAM-1 expression compared to uninfected grafts. The present experimental study shows that VAP-1 is up-regulated in acute rejection of liver allografts, and that this up-regulation is prolonged by RCMV infection.  相似文献   
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