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首页> 外文期刊>Journal of Clinical Microbiology >Use of a sensitive microplate enzyme-linked immunosorbent assay in a retrospective serological analysis of a laboratory population at risk to infection with typhus group rickettsiae.
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Use of a sensitive microplate enzyme-linked immunosorbent assay in a retrospective serological analysis of a laboratory population at risk to infection with typhus group rickettsiae.

机译:敏感的微孔板酶联免疫吸附测定法在回顾性血清分析中分析有斑疹伤寒立克次体感染风险的实验室人群。

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A microplate enzyme-linked immunosorbent assay (ELISA), developed for the detection of antibodies to typhus group rickettsiae, was used to analyze human sera from individuals engaged directly or indirectly in rickettsial research. The earliest serum available from each of 112 individuals was tested for immunoglobulin M (IgM) and IgG antibodies against Rickettsia typhi and Rickettsia prowazekii by ELISA at a 1:500 dilution. In at least one assay, nine sera had ELISA optical densities of greater than 0.2, which were above the mean optical densities plus three standard deviations of the other 103 sera. Three of the positive sera were from individuals with known clinical cases of typhus infection. The other sera with predominantly IgG titers were from individuals with extended laboratory exposure to rickettsiae or histories of typhus vaccination, or both. During continued serological surveillance, eight additional people with repeated occupational exposure to typhus rickettsiae had seroconversions in the ELISA to optical densities of greater than 0.2. No apparent clinical illness occurred in two individuals, whereas six clinical cases of infection occurred in others subsequent to accidental laboratory autoinoculation (one) or aerosol exposures (five). In the clinical infections, antibodies were first detected at 7 days, but in subsequent sera, rises and declines in titers were quite variable and were influenced by vaccination, relapse, and time and extent of antibiotic therapy. In primary infections the sera of several individuals who received immediate antibiotic therapy had brief strong IgM responses without pronounced increases in IgG. In contrast, much higher IgG levels were attained in three cases in which relapse occurred, the individual had previously been immunized, or treatment had been delayed. The microplate ELISA proved to be a highly sensitive and reliable test for detection of the human serological response to typhus antigens.
机译:为检测斑疹伤寒立克次体的抗体而开发的酶标酶联免疫吸附试验(ELISA)用于分析直接或间接参与立克次氏研究的个体的人血清。通过ELISA以1:500的稀释度测试了112个个体的最早血清中的免疫球蛋白M(IgM)和抗伤寒立克次氏体和原发立克次氏体的IgG抗体。在至少一种测定中,九种血清的ELISA光学密度大于0.2,高于平均光学密度加其他103种血清的三个标准偏差。阳性血清中的三个来自患有斑疹伤寒感染临床病例的个体。其他主要具有IgG效价的血清来自实验室长期暴露于立克次体或斑疹伤寒疫苗接种史或两者兼有的个体。在持续的血清学监测中,另外八名反复接触立克次氏菌职业的人在ELISA中的血清转化为光密度大于0.2。在两个人中没有出现明显的临床疾病,而在其他人中,有六例是由于实验室自动接种(一例)或气溶胶暴露(五例)而感染。在临床感染中,抗体是在第7天首次检测到的,但在随后的血清中,滴度的升高和降低变化很大,并受疫苗接种,复发,抗生素治疗的时间和程度的影响。在原发感染中,几名接受立即抗生素治疗的患者的血清具有短暂的强烈IgM反应,而IgG没有明显增加。相比之下,在三例复发,个体已被免疫或治疗延迟的情况下,IgG水平更高。经证明,微孔板ELISA是检测人类对斑疹伤寒抗原的血清学反应的高度灵敏且可靠的测试。

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