Prevalence and Factors Associated with Positivity of Antinuclear Antibodies (ANA) Patterns, Native Anti-DNA and Extractable Nuclear Antigens (ENA) Antibodies: Experience from a Laboratory in Dakar

Background: Diagnosis of autoimmune diseases (AID) is challenging, due to overlapping features with other non-immune disorders. Anti-nuclear antibodies (ANA) are sensitive screening tests but anti-deoxyribonucleic acid-antibody (anti-DNA), and anti-extractable nuclear antigens (anti-ENA) are specific for AIDs. We aimed to look at ANA patterns in our patients and correlated them with anti-ENA for proper interpretation and better patient management cost-effectively. Methods: A retrospective study was conducted over 1 year from January to December 2022 who were tested for ANA at biology medical laboratory of Pasteur Institute of Dakar. Anti-ENA and anti-DNA results were also analyzed for ANA-positive patients. Statistical analysis was performed using STATA 14.0, p Results: 216 patients were analyzed. Women predominated at 79.2% and mean age was 48 years [CI 95%, 46 - 50], with extremes of 10 and 89. Most represented age group was [41 - 60] with 38%. ANA was positive in 27 (12.5%) of patients, 59.2% of whom were strongly positive (titer of 1/1000, 1/3200 or 1/6400). The most common pattern was nuclear speckled, which was found in 77.8% of samples. Anti-ENA and anti-DNA positivity in ANA-positive patients was found respectively in 63% (17/27) and 1.4% (3/27) of the samples analyzed. Most commonly identified anti-ENA was anti-Sm 29.6%, anti-SSA 29.6%, anti-Ro-52 25.9%, anti-RNP 18.5% and anti-SSB 14.8% which was associated with speckled pattern. Association results indicated a significant relationship between both tests and between ANA titer in the anti-ENA- and ANA-positive patients (p 0.001). Conclusions: ANA, Anti-ENA and anti-DNA antibodies are essential for AIDS diagnosis. However, the testing repertoire should follow an algorithm comprising of clinical features, followed by ANA results with nuclear, mitotic, and cytoplasmic patterns, anti-ENA, and anti-DNA for a more meaningful, and cost-effective diagnostic approach.

Peri-nuclear antibodies correlate with survival in Greek primary biliary cirrhosis patients

AIM:To investigate possible associations of anti-nuclear envelope antibody(ANEA)with disease severity and survival in Greek primary biliary cirrhosis(PBC)patients.METHODS:Serum samples were collected at diagnosis from 147 PBC patients(85%female),who were followed-up for a median 89.5 mo(range 1-240).ANEA were detected with indirect immunofluorescence on 1% formaldehyde fixed Hep2 cells,and anti-gp210 antibodies were detected using an enzyme linked immunosorbent assay.Findings were correlated with clinical data,histology,and survival.RESULTS:ANEA were detected in 69/147(46.9%) patients and 31/147(21%)were also anti-gp210 positive.The ANEA positive patients were at a more advanced histological stage(Ⅰ-Ⅱ/Ⅲ-Ⅳ56.5%/43.5% vs 74.4%/25.6%,P=0.005)compared to the ANEA negative ones.They had a higher antimitochondrial antibodies(AMA)titer(≤1:160/>1:160 50.7%/49.3%vs 71.8%/28.2%,P=0.001)and a lower survival time(91.7 ±50.7 mo vs 101.8±55 mo,P=0.043).Moreover,they had more advanced fibrosis,portal inflammation,interface hepatitis,and proliferation of bile ductules(P =0.008,P=0.008,P=0.019,and P=0.027,respectively).They also died more frequently of hepatic failure and/or hepatocellular carcinoma(P=0.016).ANEA positive,anti-gp210 positive patients had a difference in stage(Ⅰ-Ⅱ/Ⅲ-Ⅳ54.8%/45.2%vs 74.4%/25.6%,P= 0.006),AMA titer(≤1:160/>1:160 51.6%/48.4%vs 71.8%/28.2%,P=0.009),survival(91.1±52.9 mo vs 101.8±55 mo,P=0.009),and Mayo risk score(5.5 ±1.9 vs 5.04±1.3,P=0.04)compared to the ANEA negative patients.ANEA positive,anti-gp210 negative patients had a difference in AMA titer(≤1:160/>1:160 50%/50%vs 71.8%/28.2%,P=0.002),stage(Ⅰ-Ⅱ/Ⅲ -Ⅳ57.9%/42.1%vs 74.4%/25.6%,P=0.033),fibrosis(P=0.009),portal inflammation(P=0.018),interface hepatitis(P=0.032),and proliferation of bile ductules(P=0.031).Anti-gp210 positive patients had a worse Mayo risk score(5.5±1.9 vs 4.9±1.7,P=0.038)than the anti-gp210 negative ones.CONCLUSION:The presence of ANEA and anti-gp210 identifies a subgroup of PBC patients with advanced disease severity and poor prognosis.

Appearance of an inhibitory cell nuclear antigen in rat and human serum during variable degrees of hepatic regenerative activity

AIM To determine whether proliferating cell nuclear antigen (PCNA) is present in the peripheral circulation and whether PCNA levels correlate with enhanced regenerative activity.METHODS In animal studies, adult male Sprague-Dawley rats (n=3-4/ group) were sacrificed at 0, 12, 24, 36, 48, 72 and 96 hours following 70% partial hepatectomy. At each interval, sera were analyzed by Western blot for PCNA by two monoclonal antibodies (PC-10 and 19F-4). In human studies, sera from 4 patients with liver cirrhosis and 4 healthy controls were tested in a similar manner.RESULTS The PC-10 monoclonal antibody identified a protein with a molecular mass of 120 KD which remained stable in rat sera for 24 hours following partial hepatectomy, then increased 1.5-fold at 48 hours prior to returning to baseline at 96 hours after partial hepatectomy. However, it was not detected in the sera of patients with or without liver disease. In the 19F-4 monoclonal antibody, a protein with a molecular mass of approximately 46 KD was found. which was present in rat sera prior to partial hepatectomy and for 12 hours after surgery. Thereafter, levels fell by approximately 50% at 24 hours, 65% at 36 hours and 75% at 48 hours where they remained until 96 hours after partial hepatectomy. The decrease in levels correlated with the extent of partial hepatectomy. In human sera, the appearance of this inhibitory cell nuclear antigen (ICNA) was higher in the sera of patients with cirrhosis than in healthy controls.CONCLUSION The PC-10 monoclonal antibody can detect a protein in the circulation when active hepatic regenerative activity is taking place. The 19F-4 monoclonal antibody, however, identifies a protein in both rat and human sera that inversely correlates with hepatic regenerative activity. This protein which is tentatively referred to as inhibitory cell nuclear antigen (ICNA) may be used in documenting the extent of suppression of hepatic regeneration.

HLA-B27、ANA和ANCA检测对类风湿性关节炎的诊断价值

目的探讨人类白细胞B27抗原(HLA-B27)、抗核抗体(ANA)和抗中性粒细胞胞质抗体(ANCA)在诊断类风湿性关节炎(RA)的临床价值。方法选取2018年9月至2020年9月在我院风湿科住院的患者,其中RA组132例,并随机选取同期治疗的非RA组患者132例,比较两组一般资料和维生素D(VitD)、白细胞介素33(IL-33)、白细胞介素35(IL-35)水平;分析HLA-B27、ANA和ANCA的阳性率,相关性分析IL-33、IL-35和VitD水平与HLA-B27、ANA和ANCA阳性率的关系,判断HLA-B27、ANA和ANCA诊断RA的准确性。结果两组一般资料无显著差异(P>0.05);RA组IL-33水平高于非RA组患者(P<0.05),IL-35和VitD显著低于非RA组(P<0.05);RA组HLA-B27、ANA和ANCA阳性率均高于非RA组(P<0.05);RA组患者IL-33水平与HLA-B27(+)、ANA(+)和ANCA(+)呈正相关(r=0.356、0.321和0.290,P<0.05),IL-35水平与HLA-B27(+)、ANA(+)和ANCA(+)呈负相关(r=-0.299、-0.357和-0.301,P<0.05),VitD水平与HLA-B27(+)、ANA(+)和ANCA(+)呈负相关(r=-0.407、-0.335和-0.371,P<0.05)。HLA-B27诊断RA灵敏度、特异度和kappa系数分别为77.78%、97.36%和0.697;ANA诊断RA灵敏度、特异度、和kappa系数分别为80.56%、92.68%和0.648;ANCA诊断RA灵敏度、特异度和kappa系数值分别为79.49%、95.06%和0.715;HLA-B27、ANA和ANCA联合诊断RA灵敏度、特异度和kappa系数分别为81.82%、96.00%和0.785。结论HLA-B27、ANA和ANCA联合检测可以提高RA诊断的准确度,值得临床推广使用。

ANA、抗ENA抗体联合抗ds-DNA抗体对自身免疫性疾病的诊断价值

目的 研究自身免疫性疾病诊断中抗核抗体(ANA)、抗可提取性核抗原抗体(抗ENA抗体)、抗双链DNA抗体(抗ds-DNA抗体)联合诊断的临床价值。方法 选取240例自身免疫性疾病患者为观察组,另选取240例健康体检者为对照组。两组研究对象均测定血清抗ENA抗体、ANA及抗ds-DNA抗体。对比两组血清ANA、抗ds-DNA抗体、抗ENA抗体阳性率,观察组不同疾病患者的抗ENA抗体阳性率。结果 观察组血清抗ds-DNA抗体阳性率60.42%、ANA阳性率82.08%、抗ENA抗体阳性率64.58%均显著高于对照组的0.42%、0.42%、0,差异具有统计学意义(P<0.05)。观察组不同疾病患者的抗nRNP/Sm抗体、抗Sm抗体、抗SS-A抗体、抗Ro-52抗体、抗SS-B抗体、抗SCL-70抗体、抗PM-SCL抗体、抗J0-1抗体阳性率对比,差异具有统计学意义(P<0.05)。结论 自身免疫性疾病中ANA、抗ENA抗体、抗ds-DNA抗体联合检测,可为临床诊治提供可靠依据。

抗核抗体与抗可提取性核抗原抗体联合检测对自身免疫疾病的诊断价值

目的探讨抗核抗体(ANA)与抗可提取性核抗原(ENA)抗体联合检测对自身免疫疾病的诊断价值。方法选取2018年1月至2020年9月本院收治的63例自身免疫疾病患者作为研究组,另选取同期本院60名健康体检者作为对照组,两组均进行ANA、抗ENA抗体检测。比较两组ANA阳性率,分析两组抗ENA抗体检测结果,比较研究组不同自身免疫疾病患者抗ENA抗体阳性率,分析ANA联合抗ENA抗体在自身免疫疾病中的诊断效能。结果研究组SLE、RA、SS患者ANA阳性率均高于对照组,且SLE患者高于RA及SS患者,SS患者高于RA患者,差异有统计意义(P<0.05)。研究组SLE、RA、SS患者均不同程度检出抗ENA抗体阳性,对照组抗ENA抗体检测均为阴性;研究组SLE、RA、SS患者RNP、Sm、SS-A、SS-B、Scl-70阳性率比较差异有统计学意义(P<0.05),SLE、RA、SS患者Jo-l阳性率比较差异无统计学意义;两两比较:研究组SLE患者RNP、Sm、SS-A、SS-B阳性率均高于RA患者,差异有统计学意义(P<0.05),SLE患者与RA患者Scl-70、Jo-l阳性率比较差异无统计学意义;SLE患者RNP阳性率高于SS患者,Scl-70阳性率低于SS患者(P<0.05),SLE患者与SS患者Sm、SS-A、SS-B、Jol阳性率比较差异无统计学意义;RA患者SS-A、SS-B阳性率均低于SS患者,差异有统计学意义(P<0.05),RA患者与SS患者RNP、Sm、Scl-70、Jo-l阳性率比较差异无统计学意义。绘制ROC曲线结果显示,ANA联合抗ENA抗体检测诊断自身免疫疾病的AUC为0.875,诊断价值较高;ANA联合抗ENA抗体检测诊断自身免疫疾病的灵敏度、特异度均高于ANA和抗ENA抗体单一检测(P<0.05),ANA与抗ENA抗体单一检测诊断自身免疫疾病的灵敏度、特异度比较差异无统计学意义。结论ANA与抗ENA抗体联合检测应用于自身免疫疾病患者中,可提高不同类型的自身免疫疾病自身抗体阳性检出率,具有较高的诊断价值,可为临床制订治疗方案提供准确的指导。

卵巢早衰免疫因素的相关研究

目的:探讨卵巢早衰患者抗核抗体,HLA-DR+细胞水平及定位,分析免疫因素在致病中的意义。方法:应用免疫学实验技术,流式细胞术及免疫双荧光法检测100例卵巢早衰患者,60例低促性腺激素性闭经患者,60例自然绝经妇女,60例正常育龄妇女的抗核抗体、抗双链DNA抗体、ENA多肽抗体系列、CD3+、HLA-DR+、CD3+HLA-DR+细胞水平。结果:①染色体核型正常的卵巢早衰患者抗核抗体阳性率为26.53%(26/98),染色体核型异常的卵巢早衰患者抗核抗体均为阴性。染色体核型正常的卵巢早衰患者抗核抗体阳性率均明显高于低促性腺激素组、自然绝经组、育龄组(P<0.05),未发现有明显的特殊核抗原成分;13例ANA阳性POF患者经治疗后ANA转为阴性;②卵巢早衰患者外周血HLA-DR抗原表达增加,CD3+HLA-DR+(活化T细胞)增加,与自然绝经组和育龄组比较,差异均有显著意义(P=0.001,P=0.003);6例POF患者经激素替代后CD3+HLA-DR+水平未见明显降低。结论:部分染色体核型正常的卵巢早衰患者机体存在免疫系统异常状态,免疫因素可能是染色体核型正常的卵巢早衰患者的致病原因。

低分子肝素对抗子宫内膜抗体环境中滋养细胞增殖与凋亡能力的调节作用

目的:探讨体外培养的人早孕绒毛膜滋养细胞在抗子宫内膜抗体(EmAb)环境中,低分子肝素对其增殖及凋亡能力的调节作用。方法:胰蛋白酶/DNA酶Ⅰ联合消化,通过Percoll细胞分离液纯化得到绒毛滋养细胞。按照EmAb(+)血清未加低分子肝素(A1组)、EmAb(+)血清加低分子肝素(A2组)、EmAb(-)血清未加低分子肝素(B1组)、EmAb(-)血清加低分子肝素(B2组)4个分组进行培养24h后,四甲基偶氮唑蓝比色法(MTT)检测滋养细胞细胞增殖情况,以490nm处的平均吸光度(A)值表示;采用免疫荧光化学法检测增殖细胞核抗原(PCNA)的表达水平,以平均荧光灰度值表示;采用流式细胞术检测细胞凋亡,以细胞凋亡率(%)表示。结果:(1)A1组细胞490nm处的A值为0.1007±0.0125,A2组为0.1982±0.0135,两者比较,差异有统计学意义(P<0.05);B1组细胞490 nm处的A值为0.2117±0.0106,B2组为0.2211±0.0080,两者比较,差异无统计学意义(P>0.05);(2)A1组细胞PCNA的表达水平为9.77±0.61,A2组为20.96±1.31,两者比较,差异有统计学意义(P<0.05);B1组细胞PCNA的表达水平为21.40±1.93,B2组为22.42±1.70,两者比较差异无统计学意义(P>0.05);(3)A1组细胞凋亡率为(2.64±0.10)%,A2组为(0.82±0.02)%,两者差异有统计学意义(P<0.05);B1组细胞凋亡率为(0.79±0.03)%,B2组为(0.76±0.03)%,两者差异无统计学意义(P>0.05)。结论:EmAb能抑制人早孕绒毛膜滋养细胞增殖,并促进其凋亡,这可能是导致自然流产的原因之一,而低分子肝素能够逆转这一过程。

免疫印迹法与间接免疫荧光法检测抗核抗体对照分析

目的探讨欧蒙免疫印迹法不同项目阳性与间接免疫荧光法检测抗核抗体(ANA)不同核型的相关性。方法对比分析251例欧蒙印迹法不同项目阳性病例的抗体谱类型与其ANA阳性核型。结果欧蒙印迹法抗体类型不同,ANA荧光核型有很大差别,规律不明显。结论依据荧光核型来推断抗ENA等抗体不可靠。

自身抗体检测在儿童自身免疫性疾病中的意义

目的研究抗核抗体(ANA)、ANA荧光分型、抗可溶性抗原(ENA)抗体和抗双链DNA(ds-DNA)抗体检测在儿童自身免疫性疾病中的意义。方法对住院患儿中ANA、抗ENA,或抗ds-DNA抗体至少1项阳性者共135例进行总结,分别计算其阳性预测值(PV)。结果ANA阳性中自身免疫性疾病的PV=0.36,ANA荧光强度与PV成正比,ANA荧光分型中细颗粒型对于SLE有较高的PV;抗ENA抗体和抗ds-DNA抗体对自身免疫性疾病PV高于ANA。结论ANA荧光强度,抗ENA抗体和抗ds-DNA抗体阳性对自身免疫性疾病有较高的诊断价值。

免疫印迹法检测可提取核抗原多肽抗体的评价

目的评价免疫印迹法(IB)检测可提取核抗原(ENA)多肽抗体的性能。方法以检测抗ENA抗体中的抗U1RNP抗体为研究对象,用免疫印迹法(IB)和免疫双扩散法(ID)分别进行检测,以高特异的ID法检测结果为对照,统计IB法的符合率。结果用IB法检测抗U1RNP抗体有7种不同的蛋白质排列组合,其中以73,32,17.5kDa三条蛋白带同时出现与ID法的符合率最高(84.1%),而32kDa的符合率最低(30.7%),这两组的差异最显著(P<0.01)。结论单独采用IB法检测抗ENA抗体尚欠可靠,须结合其它方法,取长补短,提高ENA抗体检测的敏感性、特异性。

Slit-Robo信号对粘液表皮样癌细胞增殖作用的影响

目的探讨Slit-Robo信号对粘液表皮样癌细胞系Mc3细胞生长与增殖作用的影响及其作用机制。方法免疫组织化学方法及流式细胞术细胞内因子检测法检测Mc3细胞Slit2及Robo1蛋白的表达;在Robo1受体胞外区的单克隆抗体R5作用下,以细胞计数法与软琼脂克隆形成实验观察Mc3细胞生长变化及用流式细胞术细胞内因子检测法检测增殖相关蛋白PCNA的表达。结果 Mc3细胞表达Slit2及Robo1蛋白,并且在R5单克隆抗体作用下,Mc3细胞体外生长能力受到抑制,增殖能力明显减弱,PCNA蛋白表达水平下降。结论 Slit-Robo信号可能影响Mc3细胞的生长增殖能力,对肿瘤细胞内的PCNA有正调控作用,提示该信号可能参与粘液表皮样癌的发生及发展过程。

自身免疫性疾病中抗核抗体与抗ENA抗体的相关性分析

目的探讨抗核抗体(ANA)荧光核型与抗可提取性核抗原抗体(ENA)之间的相关性。方法 ANA采用间接免疫荧光法检测,抗ENA抗体采用德国欧蒙公司免疫斑点法检测,检测结果采用双盲对照法分析。结果 132例抗ENA抗体阳性病例ANA的阳性率为93.9%,荧光核型主要以颗粒型为主。另外检测的103例ANA阳性病例中,抗ENA抗体常规6项阳性率为78.6%。结论抗ENA抗体类型与ANA荧光核型之间没有绝对的规律,临床检测自身抗体时需将两者结合分析。

979例自身免疫性疾病抗核抗体与抗ENA抗体联合检测的结果分析

目的回顾本实验室开展抗核抗体(antinuclear antibody,ANA)与抗可提取性核抗原(extractable nuclear antigens,ENA)抗体联合检测的情况,分析两者之间的相关性,并探讨联合检测在自身免疫性疾病中的应用价值。方法间接免疫荧光法检测ANA,生物芯片技术检测抗ENA(ds-DNA、Sm、SS-A/Ro、SS-B/La、u1RNP、Scl-70、Jo-1、RibosomalP)抗体,并采用双盲法分析ANA阳性标本的荧光核型与抗ENA抗体的关系。结果979例临床标本中,ANA阳性的标本数为400例,阳性率为40.9%(400/979)。荧光核型主要是核颗粒型(249例)、核均质型(83例)、胞浆颗粒型(30例),同时对979例标本进行抗ENA抗体的检测,阳性标本数为199例,阳性率为20.3%(199/979),只有1例阳性出现在ANA阴性的标本中。在400例ANA阳性的标本中,抗ENA抗体的阳性率为49.5%(198/400),出现较多的阳性抗体是抗SS-A/Ro(133例)、抗RibP(78例)、抗u1RNP(70例)、抗ds-DNA(61例)、抗SS-B/La(40例)等抗体,主要与颗粒型荧光相关。而均质型ANA标本中,常见的抗ENA抗体是抗ds-DNA(37例)、抗SS-A/Ro(27例)、抗Jo-1(20例)、抗RibP(20例)等抗体。结论不同荧光核型的ANA与抗ENA抗体之间的关系有各自的特点。用间接荧光法筛查ANA,并联合抗ENA抗体谱进行分型,可以确定部分ANA靶抗原的类型,进一步扩展抗ENA抗体谱,才能准确确定靶抗原。

活血化瘀药物在抗Thy-1抗体肾炎中的实验研究

目的 为了探讨活血化瘀中药在抗Thy-1抗体肾炎中的作用及其机理。方法 利用大鼠抗Thy-1抗体系膜增殖型肾炎模型,以强的松为对照,研究中药补肾活血汤、保肾康对此模型的干扰。并以免疫组化法,观察肾组织中增殖细胞核抗原(proliferating cell nuclear antigen,PCNA)的表达。结果 实验组大鼠24小时尿蛋白定量、血尿程度、肾脏病理改变及系膜区PCNA阳性细胞数的改变均较模型组明显为轻。结论补肾活血汤及保肾康对系膜增殖型肾炎有治疗作用。

血清抗可提取性核抗原抗体检测质控品的制备及评价

目的自制抗可提取性核抗原(ENA)抗体弱阳性及阴性质控品,确保常规检测工作结果的质量。方法将抗核抗体(ANA)谱阳性结果的患者血清置于56℃30min条件下灭活,离心去除沉淀后血清(结果为RNP++,Sm++,SS-A++,SS-B++,dsDNA++)与ANA及ANA谱全部阴性献血员血清按照1∶N比例混匀,配置成ENA弱阳性质控品(结果为RNP±,Sm±,SS-A±,SS-B±,dsDNA±),采用免疫印迹法和酶联免疫吸附法检测ENA弱阳性质控品,然后进行均一性、稳定性、破坏性实验验证。结果均一性、稳定性、破坏性实验验证均通过,ENA阴性质控品所有阴性的靶抗原都能够检测出阴性,所有阳性的靶抗原都能够检测出阳性。结论经过验证,ENA自制质控品符合该科要求,可以应用于常规检测工作。

抗核抗体和疱疹病毒IgG类抗体间的相关性

用ＥＬＩＳＡ间接法检测了人血清中的ＣＭＶ和ＨＳＶⅠＩｇＧ类抗体，４８份间接荧光免疫技术检测的ＡＮＡ阳性血清和５７份ＡＮＡ阴性血清，ＣＭＶＩｇＧ类抗体阳性率分别为６９％和３９％。３１份免疫印迹法检测的ＥＮＡ抗体阳性血清和６２份ＥＮＡ阴性血清，ＣＭＶＩｇＧ类抗体阳性率分别为７１％和４２％，两类抗核抗体阳性组和阴性组间ＣＭＶＩｇＧ类抗体阳性率有显著性差异，但ＨＳＶⅠＩｇＧ类抗体水平在这些抗核抗体阴性、阳性组间的差异不具显著性。

抗可提取性核抗原抗体与抗核抗体的对照分析

目的探讨抗可提取性核抗原(ENA)多肽抗体不同项目阳性时与抗核抗体(ANA)之间的相关性。方法对比分析323例抗ENA抗体(抗U1-nRNP、Sm、SS-A、SS-B、Scl-70和Jo-1抗体)阳性病例的多肽谱类型与其304例ANA阳性核型。结果抗ENA抗体类型不同,ANA荧光核型有很大差别,没有绝对的规律可言。结论不能简单地依据荧光核型来推断抗ENA抗体的具体类型。

自身抗体对乙型肝炎病毒相关性肾炎的诊断和预测价值

目的通过检测乙型肝炎病毒相关性肾炎(HBV-GN)患者血清中的自身抗体,分析自身抗体在HBV-GN中的诊断和预测价值,从而为该病的防治提供新的思路。方法对23例HBV-GN和25例乙型肝炎非肾炎患者进行病例分析,并采用间接免疫荧光法和免疫印迹法分别检测患者血清抗核抗体(ANA)和抗可溶性核抗原(ENA)抗体,比较每组抗核抗体的阳性率和核型以及抗ENA抗体谱的阳性率和种类,并对乙型肝炎非肾炎患者进行随访。结果 HBV-GN患者抗核抗体和抗ENA抗体谱阳性率显著增高,其中ANA核型以颗粒型为主,抗ENA抗体谱中Ro-52和AMA-M2居多,且自身抗体阳性的乙肝患者更易发生HBV-GN。结论自身抗体在乙型肝炎病毒相关性肾炎中有一定的检测价值,可以为疾病的预测和早期诊断提供新的参考指标。

80例狼疮肾炎病人ANA荧光核型及抗核抗体谱分析

目的探讨抗核抗体(ANA)荧光核型及抗核抗体谱多肽谱对狼疮性肾炎(LN)诊断的有效指标。方法对80例LN组、78例系统性红斑狼疮(SLE)非LN组及104例非SLE组分别用间接荧光法(IIF—ANA)和线性免疫印迹法(LIA—ANA)进行抗核抗体荧光核型、双链DNA及11项抗核抗体谱多肽谱分析。结果 LN组抗核抗体阳性率(>1∶100)为100%(80/80),LN组荧光核型均质型42.5%(34/80)显著高于非LN组21.79%(17/78)与对照组5.77%(6/104),P<0.05;LN组颗粒核型53.75%(43/80)明显低于非LN组73.08%(57/78),P<0.05。LN病例核均质型主要表现有抗Hi、Nud、dsDNA抗体,χ2为8.26、23.05、26.39(P均<0.05)。抗核抗体谱多肽谱分析,LN组仅抗dsDNA抗体55.00%(44/80)高于非LN组23.08%(18/78),差异有显著性,P<0.05。结论 SLE伴狼疮性肾炎的病人ANA荧光核型主要表现为均质型,抗dsDNA抗体阳性率显著性增高,可视为预测狼疮性肾炎的有效指标。