应用明胶凝集颗粒试验检测人群中T细胞白血病病毒抗体

曾毅等报道,应用间接免疫荧光法(IIF)检测了8,279份正常成年人血清标本,发现3例T细胞白血病病毒(HTLV)抗体阳性:一例马杨氏,丈夫是日本人(HTLV抗体也阳性),侨居南京46年;第二例是台湾籍妇女;第三例是位侨居北京的日本人。650份各类白血病病人血清中,一例成人T细胞白血病患者HTLV抗体阳性,此人是船员,常去日本。     

IDENTIFICATION OF MYCOPLASMATACEAE BY THE FLUORESCENT ANTIBODY METHOD

Clark, Harold W. (The George Washington University, Washington, D.C.), Jack S. Bailey, Richard C. Fowler, and Thomas McP. Brown. Identification of Mycoplasmataceae by the fluorescent antibody method. J. Bacteriol. 85:111-118. 1963.-The conditions of the fluorescent antibody reactions were studied in relation to their application to Mycoplasmataceae or pleuropneumonia-like organisms (PPLO). Mycoplasma hominis type 1 and 2 antigens and their homologous antisera were used to determine the activity and specificity of these and other strains. Fluorescein isothiocyanate conjugated antiserum globulin preparations were used in both the direct and indirect fluorescent antibody methods. A direct tube technique was used for the detection and measurement of growth in broth cultures by the addition of conjugated antiserum. The specific fluorescent staining and recognition of hot water fixed M. hominis colonies was presented as a suitable identification standard. The antigenic activity was found to remain in the insoluble residue after exposure of M. hominis strains to sonic vibration (9 kc) for 30 min and centrifugation. Brief 2-min exposures of tissue cells to vibration (9 kc) caused the disruption of tissues, with the release of viable and "bound" nonwashable strains that reacted specifically with fluorescent antibody. It is proposed to apply both the sonic vibration and the fluorescent antibody techniques for the identification of Mycoplasmataceae in human tissues.     

SEROLOGICAL GROUPING OF ACTINOMYCES BY MEANS OF FLUORESCENT ANTIBODIES.

Slack, John M. (West Virginia University, Morgantown), Ann Winger, and Dane W. Moore, Jr. Serological grouping of actinomyces by means of fluorescent antibodies. J. Bacteriol. 82:54-65. 1961.-Serological groups A, B, C and D of actinomyces were established using fluorescent antibody techniques. One hundred and thirty-eight cultures were included in the study. Eighty-nine were classed in group A, 15 in B, 13 in C, and 21 in D.The isolates were from patients and animals with actinomycosis and from healthy human beings. There was no correlation between source of the isolate and serological group. Furthermore, no one species could be placed exclusively in one group although the majority of those designated as Actinomyces bovis were in group A.Seventeen anaerobic diphtheroids and seven Corynebacterium acnes isolates were placed in group A. One diphtheroid was in each of groups B and D. On this basis it is suggested that these organisms be included in the genus Actinomyces.Additional species of Corynebacterium as well as Lactobacillus Propionibacterium, Streptomyces, and Nocardia did not fluoresce with any of the group antisera.     

应用ELISA法检测SARS-Ab

探讨对SAPS病毒进行临床诊断,分析ELISA法检测SARS-Ab的情况。结果显示对照组检测均为阴性,测试组发病12d前、后阳性检出率分别为2．7％、92％,总检出率为94．7％。29例疑似病人阳性检出率为31％。提示该方法敏感性、特异性强,但12d以前检出率低,而13-16d以后阳性率明显提高。     

基因重组抗原检测梅毒螺旋体抗体研究

梅毒是一种传染性很强的性传播疾病,早期诊断是防止其传播及治疗的关键。采用基因重组的梅毒螺旋体P47和P15抗原对289份临床标本进行梅毒螺旋体抗体的检测,并与常规方法进行了比较,结果表明：重组抗原ELISA法具有较高的敏感性和特异性,并能对梅毒进行早期诊断,可以代替常规方法检测梅毒螺旋体抗体。186份现患和已治愈梅毒患者标本,重组抗原ELISA法、TPHA法和RPR法均为阳性;60份健康献血员标本,重组抗原ELISA法和TPHA法、RPR法均为阴性;17份与梅毒患者有性接触者的标本,重组抗原ELISA法有2份阳性,而TPHA法、RPR法均为阴性,1个月后复查这2份血清TPHA和RPR均为阳性;6份RPR和类风湿因子均为阳性的血清,重组抗原ELISA法和TPHA法均为阴性,;20份肝硬化患者血清,3种方法检测均为阴性。     

MULTIPLEX DETECTION OF ESCHERICHIA COLI AND SALMONELLA ENTERITIDIS BY USING QUANTUM DOT-LABELED ANTIBODIES

In this study, we demonstrated the simultaneous detection of Escherichia coli and Salmonella enteritidis, by coupling immunomagnetic separation (IMS) with quantum dots (QDs) labeling. QDs having different emission wavelengths were conjugated with anti- E. coli and anti- Salmonella antibodies. QD–antibody conjugates were used to label immunomagnetically separated bacteria and the fluorescence intensities were measured for enumerations of both species. The concentrations of primary antibodies used in IMS, the ratio of QDs to antibodies during the conjugation and the concentration of QD–antibody conjugates used in labeling were optimized to enhance the sensitivity of the assay. After labeling bacteria with QDs, the quenching observed between bead–bacteria complex and QDs was eliminated by separating QDs from the complex using sodium dodecyl sulfate solution. The fluorescence intensities due to the capturing of different concentrations of bacteria were measured and the working ranges were found to be 5 × 10² to 5 × 10⁵ cfu/mL for E. coli and 4  ×  10² to 4  ×  10⁵ cfu/mL for S. enteritidis .

PRACTICAL APPLICATIONS

In this study, antibody-conjugated multicolor quantum dots (QDs) were used for simultaneous detection of Escherichia coli and Salmonella enteritidis . The results of this study indicate that QD labels can be used in multiplex, rapid and selective detection of bacteria with detection limits comparable with those of many novel methods in cases where the assay conditions are optimized. Furthermore, the assay can be modified for the simultaneous detection of more than two species through using QD labels having different emission wavelengths.     

应用ELISA法检测风疹病毒IgG抗体

实验证明,将0.1％脱氧胆酸钠制备的风疹病毒粗制抗原,用于ELISA法检测风疹病毒IgG抗体,效果较满意,方法的特异性好,与常规血凝抑制试验(HI)的相关性也好,所测抗体的几何平均值为HI的4倍。用本法初步调查了北京市不同年龄人群的风疹感染率,证明随年龄增长风疹感染率迅速上升,18岁以上人群达94％。检测河北省沧州地区孕妇的风疹IgG阳性率为99％。用於风疹病人的血清学诊断,获得较好结果。     

用抗独特型单抗体外诱发抗天花粉蛋白的二次抗体应答

在前阶段工作中已获得16个抗天花粉蛋白的单抗。用其中的一个IgE类单抗TE 1免疫Wistar大鼠,通过大鼠-小鼠杂交瘤技术得到了抗独特型单抗。现研究抗独特型单抗AId 6c5在体外诱发二次抗体应答中所起的作用。实验结果表明:1.当将AId 6c5和天花粉蛋白初次免疫8周后的小鼠脾细胞和肠系膜淋巴结细胞一起培养时,能引起二次抗体应答,说明AId 6c5能代替抗原的刺激作用,如果培养系统中同时存在AId 6c5和天花粉蛋白(其剂量能引起体外二次抗体应答),则可出现某种程度的抑制。由于AId 6c5是单克隆抗体,提示一种AId能在不同情况下起刺激或抑制作用。3.应用竞争结合试验阐明AId 6c5除和TE 1外,还和另外两个单抗——TE 4(IgE)和2 A1(IgG1)——起反应,先前的工作证明这三个单抗和另外4个单抗都识别天花粉蛋白上的同一抗原决定簇。但AId 6c5对识别这同一决定簇的其余4个单抗反应很弱。以上说明a.IgE和其它Ig类别具有共同或交叉的独特型,b.也说明识别同一决定簇的IgE具有不同的独特型。4.将TE 1等三个单抗和AId 6c5预先作用后能抑制这三个单抗和天花粉蛋白的结合,说明AId 6c5所识别的独特型,位于抗原结合部位内,至少??是很靠近抗原结合部位的。     

RT套式PCR检测血浆HCV RNA及与抗HCV检测的比较

应用微量血清热变性法提取核酸,逆转录套式聚合酶链反应(RT-nest PCR)检测血浆HCV RNA,并与抗HCV ELISA检测结果比较,对HCV RNA阳性标本进行HGV RNA的筛查.结果在32例抗HCV阳性和20例抗HCV阴性血浆中,HCV RNA分别检出18例和2例,总符合率为70%,20例HCV RNA阳性者中有2例合并感染HBV,1例合并感染HGV.证明血浆样本中抗HCV与HCV RNA间存在很大的相关性.     

应用明胶颗粒凝集试验检测人免疫缺陷病病毒(HIV-1)抗体

明胶颗粒凝集试验是测定HIV-1抗体的新方法。本研究将明胶颗粒凝集试验与ELISA法、蛋白印迹法和间接免疫荧光试验做了比较,观察本方法的敏感性和特异性。共检测了195份来自法国和非洲象牙海岸的血清,凡是蛋白印迹法阳性的血清,明胶颗粒凝试验都是阳性。这表明本方法是特异和敏感的,方法简便,不需特殊仪器,省时,可用于HIV-1抗体的筛选,但多数蛋白印迹法可疑的血清,明胶颗粒试验均阴性。因此,对蛋白印迹法测出的可疑者应该用数种方法进行追踪检测。     

UNDERSTANDING DISCRIMINATION TESTS: A USER-FRIENDLY TREATMENT OF RESPONSE BIAS, RATING AND RANKING R-INDEX TESTS AND THEIR RELATIONSHIP TO SIGNAL DETECTION

Aproblem central to sensory difference testing is response bias. There are two experimental strategies for dealing with this problem. The first is to use forced choice procedures, like the common duo-trio or triangle tests, while the second is to use signal detection measures like d′, P(A) and the R-index. These strategies are explained and discussed. The relationship between the R-index and the other signal detection measures is explained. The relationship between R-index values obtained by rating and ranking is explored, as are the alternative computations of the R-index by ranking: R_jb and R_mat.     

分泌人体肝癌单克隆抗体的两个小鼠杂交瘤株及其抗体的专一性分析(简报)

有证据表明人体肝癌细胞表面膜抗原的成份与正常肝细胞的有差异。应用125I UdR释放试验也证明肝癌患者的周围血淋巴细胞对体外培养的肝癌细胞有细胞毒作用。表明患者的免疫系统有可能识别这些膜抗原的差异性。但除了与人体肝癌有交义反应的胚胎肝抗原的性质有些初步报道以外,人体肝癌相关抗原的种类     

ELISA间接法检测呼吸道合胞病毒和副流感病毒血清IgM和IgA抗体

建立了检测呼吸道合胞病毒(RSV)和副流感病毒(PFV)血清特异性IgM和IgA抗体的间接ELISA方法。在方法统一的基础上比较了检测IgG、IgM和IgA抗体的结果,证明检测血清IgM和IgA可以作为RSV和PFV感染的早期诊断指标。检测了120份临床急性下呼吸道感染患儿的血清,RSV-IgM检出率为33.3％,RSV-IgA为36.7％;PFV-IgM为27.5％,PFV-IgA为31.6％。提出了对RSV和PFV感染以检测特异性IgA替代IgM或两者互补的设想。     

hTERT基因片段的克隆、表达和抗hTERT抗体用于端粒酶及hTERT检测的研究

端粒酶是一种重要的肿瘤生物学标志,其活性在生殖细胞、绝大多数肿瘤细胞和体外培养的永生细胞可以测知,但在大多数体细胞中不易测出。人端粒酶由两部分组成,包括hTERC和hTERT,hTERC在正常细胞和肿瘤细胞中均有表达,而hTERT的表达似乎受到严格的调控且和端粒酶活性一致。为了检测肿瘤细胞中端粒酶及hTERT的表达,我们制备了抗hTERT蛋白的特异性多克隆抗体。首先用RT-PCR方法克隆了hTERTcDNA的一个片段,将其连接到GST融合表达载体pGEX-5X-3后在大肠杆菌中融合表达。将纯化的融合蛋白抗原免疫动物,制备抗hTERT蛋白的多克隆抗体。不同的细胞抽提物用该抗体进行了Westernblot分析,结果表明该抗体可特异识别端粒酶阳性细胞株中的hTERT及端粒酶,为端粒酶及hTERT的检测初步提供了一个简单有效的检测手段。