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使用全血在艾滋病临床试验中测量诱导细胞因子:初步报告。艾滋病临床试验组诱导细胞因子焦点小组。艾滋病临床试验组。

Measurement of induced cytokines in AIDS clinical trials using whole blood: a preliminary report. ACTG Inducible Cytokines Focus Group. AIDS Clinical Trials Group.

作者信息

Wallis R S, Lederman H M, Spritzler J, Devers J L, Georges D, Weinberg A, Stehn S, Lederman M M

机构信息

Department of Medicine, University Hospitals and CWRU School of Medicine, Cleveland, Ohio 44106-4984, USA.

出版信息

Clin Diagn Lab Immunol. 1998 Jul;5(4):556-60. doi: 10.1128/CDLI.5.4.556-560.1998.

Abstract

Measures of immune function have become increasingly important as endpoints in AIDS clinical trials, with respect to both modulation and reconstitution of immunity by experimental therapies. Measurement of immune function in this setting requires the development of robust analytic approaches suitable for the clinical laboratory. Experiments were performed to evaluate the suitability of using cultured heparinized ("whole") blood for induction of tumor necrosis factor alpha (TNF-alpha) and gamma interferon (IFN-gamma), two cytokines critical in AIDS pathogenesis. TNF-alpha expression ranged from 229 to 769 pg/ml in lipopolysaccharide (LPS)-stimulated cultures and was not detected in unstimulated cultures. IFN-gamma expression ranged from 0 to 112,000 pg/ml in phytohemagglutinin A (PHA)-stimulated cultures and from 0 to 789 pg/ml in antigen-stimulated cultures. The mean coefficient of variation observed in three weekly determinations was 0.47 for TNF-alpha and ranged from 0.12 to 1.73 for IFN-gamma. These values indicate that sample sizes of 8, 24, and 29 subjects would be sufficient to detect twofold changes in LPS-induced TNF-alpha and in PHA- and antigen-induced IFN-gamma respectively, if two baseline and two treatment determinations were obtained, and if the interpatient variability of changes in true levels from baseline to follow-up is negligible compared to the variability in the three weekly measurements. Measurement of LPS-induced TNF-alpha and mitogen- or antigen-induced IFN-gamma can be performed simply and reproducibly in human immunodeficiency virus-infected persons by the whole-blood culture method. Further studies are warranted to determine the effect of overnight shipping on assay reproducibility and to determine the extent to which responses can be reliably detected in subjects with low CD4 cell numbers.

摘要

免疫功能的检测作为艾滋病临床试验的终点变得越来越重要,这涉及到实验性疗法对免疫的调节和重建。在这种情况下,免疫功能的检测需要开发适用于临床实验室的可靠分析方法。进行了实验以评估使用培养的肝素化(“全”)血诱导肿瘤坏死因子α(TNF-α)和γ干扰素(IFN-γ)的适用性,这两种细胞因子在艾滋病发病机制中至关重要。在脂多糖(LPS)刺激的培养物中,TNF-α表达范围为229至769 pg/ml,在未刺激的培养物中未检测到。在植物血凝素A(PHA)刺激的培养物中,IFN-γ表达范围为0至112,000 pg/ml,在抗原刺激的培养物中为0至789 pg/ml。在每周三次的测定中观察到的平均变异系数,TNF-α为0.47,IFN-γ为0.12至1.73。这些值表明,如果获得两次基线和两次治疗测定,并且与三次每周测量的变异性相比,从基线到随访的真实水平变化的患者间变异性可忽略不计,那么分别有8、24和29名受试者的样本量足以检测LPS诱导的TNF-α以及PHA和抗原诱导的IFN-γ的两倍变化。通过全血培养方法可以在人类免疫缺陷病毒感染的个体中简单且可重复地进行LPS诱导的TNF-α以及有丝分裂原或抗原诱导的IFN-γ的检测。有必要进一步研究以确定隔夜运输对检测重现性的影响,并确定在低CD4细胞数的受试者中能够可靠检测到反应的程度。

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