新生儿溶血病ABO血型免疫性抗体检测分析

目的探讨分析新生儿溶血病(Hemolytic Disease of the Newborn, HDN)ABO血型免疫性抗体检测的价值。方法选取我院2011年1月~2013年12月期间收治的200例新生儿高胆红素血症患儿,采用抗人球蛋白法和微柱凝胶法对患儿实施血型血清学检测,对于母婴ABO血型系统不合的HDN患儿的血液标本进行新生儿溶血三项检验院直接Coomb实验、游离抗体测定、抗体释放实验,检测免疫性抗体IgG的特异性。结果200例新生儿高胆红素血症患儿中,母婴ABO血型系统不合的HDN发生率为56﹪(112/200)。母婴ABO血型系统不合的HDN患儿中,48.21﹪(54/112)的患儿为IgG抗A导致,51.79﹪(58/112)的患儿为IgG抗B导致。其中直接Coomb实验的阳性率为36.61﹪(41/112),游离抗体测定的阳性率为79.46﹪(89/112),抗体释放实验的阳性率为100﹪(112/112)。结论新生儿溶血病ABO血型免疫性抗体检测的价值较大,能够快速有效的诊断,因此及时采取有效的治疗,对防治HDN具有重要意义。

自身免疫性抗体检测在肝病诊断中的价值探讨

目的探讨肝病诊断采取自身免疫性抗体检测的临床价值。方法选取大同市第五人民医院2015年4月—2019年11月收治的自身免疫性肝病患者118例,依照病理性质分为自身免疫性肝炎组(AIH,n=53)原发性胆汁性肝硬化组(PBC,n=65)2个亚组;选择同期85例病毒性肝炎患者,依照病理性质分为乙型病毒性肝炎组(HBV,n=48)丙型病毒性肝炎组(HCV,n=37)2个亚组。对4组患者采用线性免疫分析法检测自身抗体,并对检测结果进行统计分析,探讨自身抗体检测在肝病诊断中的价值。结果 AIH组中共检出自身免疫抗体阳性者31例,检出率为58.5%;PBC组中共检出60例自身抗体阳性者,检出率为92.3%,均明显高于HBV、HCV组的0.0%(P<0.05)。结论自身免疫性抗体检测可以对肝病不同类型进行有效区分,对临床诊断、治疗方案的制定及预后判断均有重要意义,值得进一步深入研究。

自身免疫性肝病抗体谱检测在自身免疫性肝病中的诊断价值

目的探讨自身免疫性肝病(ALD)抗体谱检测在ALD中的诊断价值。方法回顾性分析2018年1月至2019年12月大庆市第三医院收治的74例ALD患者的临床资料,按疾病类型的不同分为原发性胆汁性胆管炎(PBC)组36例和自身免疫性肝炎(AIH)组38例,另选取同期健康志愿者35例的体检资料,作为对照组。3组研究对象均进行ALD抗体谱检测。比较3组研究对象ALD抗体谱阳性检出率;比较AIH不同亚型ALD抗体谱阳性检出率;ROC曲线分析ALD抗体谱检测对PBC、AIH的诊断效能。结果 PBC组、AIH组ALD抗体谱检测显示,研究对象阳性率均高于对照组;PBC组中AMA-M2、gp-210阳性检出率高于AIH组、对照组;AIH组中LC-1、LKM-1阳性检出率高于PBC组、对照组;AIH-Ⅰ亚型患者中LC-1阳性检出率高于AIH-Ⅲ亚型;AIH-Ⅱ亚型患者中LKM-1阳性检出率高于AIH-I、AIH-Ⅲ亚型;AIH-Ⅲ亚型患者中SLA/LP阳性检出率高于AIH-Ⅰ亚型、AIH-Ⅱ亚型(均P<0.05),AIH-Ⅰ亚型以LC-1、AMA-M2抗体检测为主;AIH-Ⅱ亚型以LC-1、LKM-1抗体检测为主;AIH-Ⅲ亚型以SLA/LP、SP100抗体检测为主;PBC组ALD抗体谱检测中AMA-M2诊断的灵敏度与特异性最高(58.33%,85.00%);AIH组ALD抗体谱检测中LC-1诊断的灵敏度最高(52.63%)、LKM-1诊断的特异度最高(100.00%)(均P<0.05)。结论 ALD抗体谱检测利于ALD患者早期诊断,帮助ALD患者进行分型鉴别,具有较高的诊断价值。

自身免疫性抗体检测在肝病诊断中的应用效果

目的探讨自身免疫性抗体检测在肝病诊断中的应用效果。方法选取2018年1月至2020年1月于本院检查治疗的94例肝病患者作为研究对象,按照病情分为观察组(自身免疫性肝病,n=62)和对照组(其他肝病,n=32)。两组均进行自身免疫性抗体检测和肝功能指标检测,比较两组自身免疫性抗体水平和肝功能指标。结果观察组天冬氨酸转氨酶、血清丙氨酸转氨酶、碱性磷酸酶、谷氨酰转肽酶、免疫球蛋白水平均高于对照组,差异有统计学意义(P<0.05)。观察组自身免疫性抗体阳性检出率为69.35%,高于对照组的0.00%,差异有统计学意义(P<0.05);观察组抗核抗体阳性率为59.67%,明显高于对照组的37.50%,差异有统计学意义(P<0.05)。结论自身免疫性抗体检测能准确诊断自身免疫性肝病,可区别于其他肝脏疾病,为制订治疗方案提供可靠的数据支持,具有较高的临床应用价值。

新生儿溶血病红细胞血型免疫性抗体的特异性分析

目的:观察母婴血型不合新生儿溶血病(HDN)红细胞血型免疫性抗体的检出率及其特异性。方法:采用试管法和微柱凝胶法对母婴血标本进行ABO、Rh血型鉴定及不规则抗体筛查,对有黄疸症状的新生儿血标本进行直接抗人球蛋白试验、抗体游离试验、抗体放散试验、抗体特异性鉴定及其效价测定。结果:在298例由红细胞血型免疫性抗体引起的HDN患儿中,检出抗A62例(20.8%),抗B65例(21.8%),抗A+抗AB87例(29.2%),抗B+抗AB6例(2.0%);抗M4例(1.3%),抗N1例(0.3%);抗D4例(1.3%),抗E7例(2.3%),抗cE3例(1.0%)。由ABO及MN血型免疫性抗体引起HDN者,直接抗人球蛋白试验多为弱阳性,由Rh血型免疫性抗体引起HDN者,直接抗人球蛋白试验多为强阳性;微柱凝胶法的凝集强度高于试管法;HDN患儿出生后24h内阳性检出率为91.5%。结论:HDN血型免疫性抗体的特异性主要为ABO系统的抗A、抗B、抗AB,其次为Rh系统的抗E、抗D、抗cE及MN系统的抗M、抗N。

小反刍兽疫病毒H基因在杆状病毒中的表达及其免疫原性研究

为表达小反刍兽疫病毒(PPRV)H蛋白,并探讨其免疫原性,通过RT-PCR克隆PPRV Nigeria75/1毒株H基因,将其克隆至供体质粒pFB-LIC-Bse中,测序验证后将重组质粒pFB-LIC-Bse-PPRV-H转化至DH10Bac感受态细胞中,经同源重组获得重组杆状病毒穿梭质粒bacmid-PPRV-H,将其转染昆虫细胞sf21获得含有PPRV H基因的重组杆状病毒。采用SDS-PAGE、Western blot、IFA及小鼠免疫试验鉴定表达产物的反应原性及免疫原性。结果表明,在杆状病毒表达系统中表达的PPRV H蛋白能与His-tag单克隆抗体及PPRV阳性血清发生特异性反应,其相对分子质量为68ku;表达产物接种小鼠可诱导其产生特异性抗体和抗小反刍兽疫病毒中和抗体,淋巴细胞增殖试验检测结果表明重组杆状病毒rBacmid-H能与相应抗体和致敏的效应淋巴细胞发生较强的特异性反应。本试验获得的重组杆状病毒表达的PPRV H蛋白具有良好的免疫原性及反应原性,可诱导小鼠产生保护性中和抗体,该试验为进一步开发小反刍兽疫亚单位疫苗奠定了基础。

阴性选择算法检测器生成的优化及仿真

针对现有常规阴性选择算法在非我空间覆盖设计上未考虑自身免疫性检测器发生的问题,提出一种能检测和剔除自身免疫性检测器的方法,并以MATLAB软件为仿真实验平台,分别对不规则分布数据、环形分布数据和近圆形分布数据3种空间数据分布进行仿真研究.仿真结果表明,该方法能有效剔除90%的自身免疫性检测器,提升了免疫阴性选择算法的鲁棒性和自适应能力.

618例不孕患者血清免疫学抗体检测及临床意义

目的探究血清免疫学抗体检测及临床意义。方法选取2012年1月-2014年1月期间在南阳市人口和计划生育指导中心接受治疗自然流产、原发不孕、继发不孕者618例。采用酶联免疫吸附法对618例患者的血清进行抗体检测,并分析检测结果。结果 618例患者中84例AoAb抗体阳性,154例EmAb抗体阳性,163例AsAb抗体阳性,86例AcAAb抗体阳性,49例ZPAb抗体阳性,82例HgGAb抗体阳性。618例患者中有183例原发不孕患者,343例继发不孕患者和92例自然流产患者。两两比较3组患者、EmAb阳性、AcAAb阳性、AoAb阳性、HcAAB阳性、TAAb阳性差异具有统计学意义(P<0.05)。结论在不孕患者中AsAb阳性所占比例最高,在自然流产、原发性不孕和继发不孕患者中AcAAb阳性、AoAb阳性和EmAb阳性所占比例最高。这些自身抗体表达异常增大了育龄妇女的不孕发生率,因此应当给予不孕不育患者血清免疫学抗体检测,以寻找造成其不孕不育的原因,为临床治疗提供依据。

Induction of Endothelial Cell Apoptosis by Anti-alpha-enolase Antibody

Objective To assess the prevalence of anti-alpha-enolase antibody in systemic autoimmune diseases in Chinese patients and its role in endothelial cell apoptosis.Methods The reactivity of anti-alpha-enolase antibody in a variety of autoimmune disorders in Chinese patients was evaluated by dot blot assay.Endothelial cell apoptosis was investigated by in vitro incubation of endothelial cells with IgG purified from anti-alpha-enolase antibody-positive sera,with or without pre-incubation with recombinant alpha-enolase.Results Anti-alpha-enolase antibody was prevalent in different systemic autoimmune diseases with relatively high reactivity in Chinese patients.In vitro incubation of endothelial cells with IgG containing anti-alpha-enolase antibody induced apoptosis in a time-and dose-dependent manner.Apoptosis was partly inhibited by pre-incubation of the endothelial cells with recombinant alpha-enolase.Conclusions Our data suggest that alpha-enolase is a common auto-antigen recognized by anti-endothelial cell antibodies in connective tissue disease.Interaction between alpha-enolase and its autoantibody plays a role in endothelial cell apoptosis.Changes other than cell killing may contribute to the pathogenesis of endothelial damage and microvascular lesions.

Correlation of p53 over-expression and alteration in p53 gene detected by polymerase chain reaction-single strand conformation polymorphism in adenocarcinoma of gastric cancer patients from India

AIM： To study the alterations in p53 gene among Indian gastric cancer patients and to correlate them with the various clinicopathological parameters. METHODS： A total of 103 gastric cancer patients were included in this study. The p53 alterations were studied by both immunohistochemical method as well as polymerase chain reaction （PCR）-single strand conformation polymorphism （SSCP） analysis. We only studied four （exon 5, 6, 7, and 8） of the 11 ,p53 exons. The alterations in p53 were also correlated with respect to various clinicopathological parameters. RESULTS： Among 103 cases, p53 over-expression and alteration were detected in 37 （35.92%） and 19 （18.44%） cases, respectively. Most of the ,p53 alterations were found at exon 5 （31.54%）, followed by exon 6 （26.31%）, exon 7 （21.04%） and exon 8 （21.04%）. A significant correlation of p53 overexpression was found with p53 alteration （P = 0.000）. Concordance between ,p53 alteration （as detected by SSCP） and over-expression [as detected by immunohistochemistry （IHC）] was found in 75% cases. We found that IHC-positive/SSCP-negative cases accounted for 21% of cases and IHC-negative/SSCP- positive cases accounted for remaining 4% cases. CONCLUSION： Our results show that p53 gene mutations are significantly correlated with p53 protein over-expression, with 75% concordance in over-expression and alteration in the p53 gene, but 25% disconcordance also cautions against the assumption that p53 over-expression is always associated with a gene mutation. There may be other mechanisms responsible for stabilization and accumulation of p53 protein with no evidence of gene mutation that reflect an accumulation of a non-mutated protein, or a false negative SSCP result.

Helicobacter pylori-negative Russell body gastritis:Case report

Russell body gastritis is an unusual form of chronic gastritis characterized by the permeation of lamina propria by numerous plasma cells with eosinophilic cytoplasmic inclusions.Very few cases have been reported in the literature;the majority of which have shown Helicobacter Pylori(H.pylori)infection,thus suggesting a correlation between plasma cell presence and antigenic stimulation by H.pylori.We present a case of Russell body gastritis in a 78-year-old woman who was undergoing esophagogastroduodenoscopy for epigastric pain.Gastric biopsy of the gastroesophageal junction showed the presence of cells with periodic acid-Schiff-positive hyaline pink bodies.Giemsa staining for H.pylori infection was nega-tive,as well as immunohistochemical detection.The cells with eosinophilic inclusions stained positive for CD138,CD79a,andκand lambda light chains,which confirmed plasma cell origin.In particular,κand lambda light chains showed a polyclonal origin and the patient was negative for immunological dyscrasia.The histological observations were confirmed by ultrastructural examination.The cases reported in the literature associated with H.pylori infection have shown regression of plasma cells after eradication of H.pylori.Nothing is known about the progression of H.pylori-negative cases.The unusual morphological appearance of this type of chronic gastritis should not be misinterpreted during routine examination,and it should be distinguished from other common forms of chronic gastritis.It is mandatory to exclude neoplastic diseases such as gastric carcinoma, lymphoma and plasmocytoma by immunohistochemistry and electron microscopy,which can help with differential diagnosis.The long-term effects of plasma cells hyperactivation are still unknown,because cases of gastric tumor that originated in patients affected by Russell body gastritis have not been described in the literature.We are of the opinion that these patients should be scheduled for endoscopic surveillance.

Reliability of a Tissue Microarray in Detecting Thyroid Transcription Factor-1 Protein in Lung Carcinomas

OBJECTIVE To compare the expression of the thyroid transcription factor-1 （TTF-1） in human normal adult type Ⅱ alveolar epithelial cells, embryonic pneumocytes and cancer cells of lung carcinoma and metastatic lymph nodes using a tissue microarray （TMA） along with paired conventional full sections, and to investigate the reliability of tissue microarrays in detecting protein expression in lung carcinoma. METHODS A lung carcinoma TMA including 765 cores was constructed. TTF-1 protein expression in both TMA and paired conventional full sections were detected by the immunohistochemical SP method using a monoclonal antibody to TTF-1. A PU （Positive Unit） of TTF-1 protein was assessed quantitatively by the Leica Q500MC image analysis system with results from the paired conventional full sections as controls. RESULTS There was no significance between TMA and paired conventional full sections in TTF-1 expression in different nuclei of the lung tissue. CONCLUSION TTF-1 protein expression in lung carcinoma detected by TMA was highly concordant with that of paired full sections. TMA is a reliable method in detecting protein expression.

Colorectal cancer screening: Comparison of transferrin and immuno fecal occult blood test

AIM: To evaluate the sensitivity and specificity of transfesrrin dipstick test (Tf) in colorectal cancer (CRC) screening and precancerous lesions screening. METHODS: Eight hundreds and sixty-one individuals at high-risk for CRC were recruited. Six hundreds and eleven subsequently received the three fecal occult blood tests and colonoscopy with biopsy performed as needed. Fecal samples were obtained on the day before colonoscopy. Tf, immuno fecal occult blood test (IFOBT) and guaiac fecal occult blood test (g-FOBT) were performed simultaneously on the same stool. To minimize false-negative cases, all subjects with negative samples were asked to provide an additional stool specimen for a second test even a third test. If the results were all negative after testing three repeated samples, the subject was considered a true negative. The performance characteristics of Tf for detecting CRC and precancerous lesions were examined and compared to those of IFOBT and the combination of Tf, IFOBT and g-FOBT. RESULTS: A total of six hundreds and eleven subjects met the study criteria including 25 with CRC and 60 with precancerous lesions. Sensitivity for detecting CRC was 92% for Tf and 96% for IFOBT, specificities of Tf and IFOBT were both 72.0% (95% CI: 68.2%-75.5%; χ2 = 0.4, P > 0.05); positive likelihood ratios of those were 3.3 (95% CI: 2.8-3.9) and 3.4 (95% CI: 2.9-4.0), respectively. In precancerous lesions, sensitivities for Tf and IFOBT were 50% and 58%, respectively (χ 2 = 0.8, P > 0.05); specificities of Tf and IFOBT were 71.5% (95% CI: 67.6%-75.1%) and 72.2% (95% CI: 68.4%-75.8%); positive likelihood ratios of those were 1.8 (95% CI: 1.3-2.3) and 2.1 (95% CI: 1.6-2.7), respectively; compared to IFOBT, g-FOBT+ Tf+ IFOBT had a significantly higher positive rate for precancerous lesions (83% vs 58%, respectively; χ 2 = 9.1, P < 0.05). In patients with CRC and precancerous lesions, the sensitivities of Tf and IFOBT were 62% and 69% (χ 2 = 0.9, P > 0.05); specificities of those were 74.5% (95% CI: 70.6%-78.1%) and 75.5% (95% CI: 71.6%-79.0%); positive likelihood ratios of those were 2.5 (95% CI: 2.0-3.1) and 2.8 (95% CI: 2.3-3.5). Compared to IF-OBT alone, combining g-FOBT, IFOBT and Tf led to significantly increased sensitivity for detecting CRC and cancerous lesions (69% vs 88%, respectively; χ 2 = 9.0, P < 0.05). CONCLUSION: Tf dipstick test might be used as an ad- ditional tool for CRC and precancerous lesions screening in a high-risk cohort.

Glycation of high-density lipoprotein triggers oxidative stress and promotes the proliferation and migration of vascular smooth muscle cells

Background In type 2 diabetes mellitus （T2DM）, high-density lipoprotein （HDL） impairs its anti-atherogenic properties and even develops to a pro-inflammatory and pro-atherogenic phenotype because of abnormal compositions and modifications. In this study, we ex- amined the effects and the related mechanisms of glycation of HDL on the proliferation and migration of vascular smooth muscle cells （VSMCs）. Methods ＆ Results Glycated HDL （G-HDL） was modified with D-glucose （25 mmol/L） in vitro. Diabetic HDL （D-HDL） was isolated from T2DM patients. Rat VSMCs were isolated from the thoracic aortas. Human VSMCs were obtained from ScienCell Research Laboratories. Alpha-actin was detected through immunofiuorescence. VSMC proliferation was assayed by Cell Count. VSMC migration was determined by transwell chamber and scratch-wound assay. Intracellular reactive oxygen species （ROS） was detected based on ROS-medi- ated 2＇,7＇-dichlorofluorescein （DCFH-DA） fluorescence. Compared to native HDL （N-HDL）, G-HDL remarkably promoted VSMC prolif- eration and migration in the dose and time-dependent manners. In addition, G-HDL enhanced ROS generation in VSMCs. However, the ROS scavenger, N-acetylcysteine, efficiently decreased ROS production and subsequently inhibited the proliferation of VSMCs induced by G-HDL. Similarly, D-HDL from T2DM patients also promoted ROS release and VSMC proliferation and migration. Conclusions HDL either glycated in vitro or isolated from T2DM patients triggered VSMC proliferation, migration, and oxidative stress. These results might partly interpret the higher morbidity of cardiovascular disease in T2DM patients.

Development of a Fast ELISA for the Specific Detection of both Leucomalachite Green and Malachite Green

Malachite green(MG), a dye, is an antifungal agent that has been used to treat and prevent fish diseases. It is metabolized into reduced leucomalachite green forms(LMG) that may reside in fish muscles for a long period, thus being harmful to human health. The aim of this study was to develop a competitive and direct enzyme-linked immunosorbent assay(ELISA) to detect MG and LMG specifically. The monoclonal antibody(m Ab) to LMG was generated using a hybridoma technique. The obtained m Ab showed good cross-reactivity(CR) to malachite green(MG), but not to crystal violet(CV) and Brilliant Green(BG). The m Ab was used to develop a fast detecting ELISA of MG and LMG in fish. By introducing the conjugation LMG-HRP, the detection capability was 0.37 ng m L-1 for MG and LMG. The mean recovery from spiked grass carp tissues ranged from 76.2% to 82.9% and the coefficients of variation varied between 1.8% and 7.5%. The stable and efficient monoclonal cell line obtained is a sustainable source of sensitive and specific antibody to MG and LMG.

The expression and clinical significance of BRAF in prostate cancer

Objective:The aim of this study was to investigate the expression of BRAF of prostate cancer,and to explore its relations with clinic-pathological factors.Methods:Immunohistochemistry was used to detect the expression of BRAF in 74 cases of prostate cancer,and 51 cases of benign prostate hyperplasia(BPH).Results:The positive rate of BRAF had significant difference between patients with prostate cancer and BPH(P < 0.05).The expression of BRAF was correlated with grade and stage of prostate cancer(P < 0.05),but not to age of onset(P > 0.05).Conclusion:The expression of BRAF may play a role in the tumorigenesis and progression of colorectal cancer.BRAF could be a factor to diagnose the typing of prostate cancers and predict the prognosis of prostate cancers.

Expression of Hsp70 and Caspase-3 in rabbits after se- vere traumatic brain injury

Objective： To investigate the expres- sion of Caspase-3 and Hsp70 in rabbits after severe trau- matic brain injury （TBI） and to explore the feasibility of its application in estimation of injury time in forensic medicine. Methods： Arabbit model of heavy TBI was developed by high velocity impact on the parietal bone with an iron stick. Totally 8 healthy adult New Zealand white rabbits were randomly divided into control group （n=2） and injury group （n=6）. Four hours after injury, tissue specimens from the parietal lobe, temporal lobe, occipital lobe, cerebellum and brainstem were harvested to detect the expression of Hsp70 and Caspase-3 by immunohistochemistry. Besides, the gray values of cells positive for HspT0 and Caspase-3 were analyzed with an image analyzer. Results： Immunohistochemistry staining demonstrated a low level of Caspase-3 and Hsp70 expression in normal control group. While in injury group, both the Caspase-3 and Hsp70 expression was significantly elevated （P〈0.05）. Positive cells gathered around the lesion focus. Occipital lobe and cerebellum had fewer positive cells while temporal and brainstem had the fewest. Conclusion： The expression of Caspase-3 and HspT0 at an early stage following severe TBI is characteristic and can be applied to estimate the time of injury.