Seropositivity rates of water channel protein 4 antibodies compared between a cell-based immunofluorescence assay and an enzyme-linked immunosorbent assay in neuromyelitis optica patients

A total of 66 samples （from 27 cases with neuromyelitis optica, 26 cases with multiple sclerosis, aa 13 cases with optic neuritis） were tested for aquaporin-4 antibody by a cell-based immunofluorescence assay and an enzyme-linked immunosorbent assay. The sensitivities and specificities of the two assays were similar. We further analyzed an additional 68 patients and 93 healthy controls using the enzyme-linked immunosorbent assay. A Kappa test showed good consistency between the two methods in terms of detection of anti-aquaporin-4 antibody in the se of neuromyelitis optica patients. No significant correlations were identified with onset age or disea duration, suggesting that aquaporin-4 antibody is a good marker for neuromyelitis optica. The enzyme-linked immunosorbent assay can be used for quantifying aquaporin-4 antibody concentrations and may be useful to dynamically monitor changes in the levels of aquaporin-4 antibody during disease duration.

Determination of anti-endomysium IgA antibodies in the diagnosis of celiac disease:Comparison of a novel ELISA-based assay with conventional immunofluorescence

AIM： To evaluate the novel anti-endomysium （anti-EMA） detection based on ELISA. METHODS： Anti-EMA IgA was measured by a novel ELISA in 196 patients with gastrointestinal symptoms and suspected mal-absorption. Data were compared with those obtained by the conventional IF test. RESULTS： A good concordance of 98% was found between these two assays. In sera of 161 patients （82%） both assays tested negative whereas in sera of 31 patients （16%） both assays tested positive for the presence of anti-EMA antibodies. Discrepancies between EMA- ELISA and EMA-immunofluorescence （IF） were found in only 4 patients （2%）.CONCLUSION： This ELISA can replace IF for the detection of anti-EMA antibodies and provide clinicians with an excellent tool to screen for celiac disease in patients with gastrointestinal complaints.

Immunofluorescence on paraffin embedded renal biopsies:Experience of a tertiary care center with review of literature

AIMTo describe the technique of immunofluorescence on paraffin embedded tissue sections and discuss the po-tential pitfalls with an in depth review of literature.METHODSImmunofluorescence is integral to diagnostic renal pa-thology. Immunofluorescence on paraffin embedded renal biopsies （IF-P） after enzyme treatment has been described in literature, however has not found widespread use in renal pathology laboratories. In our laboratory proteinase K digestion of paraffn embedded renal biopsy material was standardized and applied prospectively in cases where immunofuorescence on fresh frozen tissue was non contributory or not possible. Diagnostic utility was assessed and in a cohort of cases comparison of intensity of staining with routine immunofuorescence was performed.RESULTSOver the 5-year study period, of the 3141 renal biopsies received IF-P was performed on 246 cases （7.7%） and was interpretable with optimal digestion in 214 cases （6.8%）. It was of diagnostic utility in the majority of cases, which predominantly included glomerular disease. Non-diagnostic IF-P was found in membranous nephropathy （2 of 11 cases）, membranoproliferative glomerulonephritis （2 of 32 cases）, lupus nephritis （1 of 25 cases）, post infectious glomerulonephritis （1 of 11 cases） and chronic glomerulonephritis （3 of 8 cases）. Comparing cases with both routine IF and IF-P, 35 of 37 showed either equal intensity or a minor difference in intensity of staining（1＋） for the diagnostic immunoglobulin/complement. Technically assessment of immunofluorescence on the paraffin embedded tissue was found to be easier with clearly observed morphology, however a false positive staining pattern was observed in under-digested tissue. CONCLUSIONAs a “salvage” technique, immunofuorescence on paraffn embedded renal biopsies is of great diagnostic utility, however not without pitfalls.

COMPARISON BETWEEN IMMUNOFLUORESCENCE AND PCR IN DETECTING HUMAN PAPILLOMA VIRUS IN CONDYLOMA ACUMINATA

Objective To compare the effectiveness of immunofluorescence and polymerase chain reaction （PCR） in detecring human papilloma virus （HPV） in condyloma acuminata （CA）. Methods HPVs in CA tissues from 60 patients were detected by immunofluorescence and PCR, respectively. Different subtypes of HPVs were also identified with restriction fragment length polymorphism （RFLP） . Resuits The positive detective rates of immunofluorescence and PCR were 56. 67 % （34/60） and 96. 67 % （58/ 60）, respectively （ P 〈 0. 01 ）. RFLP results showed HPV6 and HPV11 were the main subtypes in the detected virus, which accounted for 98.28%. Conclusion The sensibility of PCR is superior to that of immunofluorescence.

The Application of Quantum Dots Double-Labeling Immunofluorescence Technology in Detection of PR and CD146 in Paraffin-Embedded Tissue Sections of Endometrioid Adenocarcinoma

Objective: The aim was to detect the expression of PR and CD146 in paraf-fin-embedded tissue sections of endometrioid adenocarcinoma by using QDs double-labeling immunofluorescence, and evaluate the applied value of QDs double-labeling immunofluorescence in endometrioid adenocarcinoma. Methods: To detect the expression of PR and CD146 on 140 cases of paraffin-embedded tissue sections of endometrioid adenocarcinoma by using QDS double-labeling immunofluorescence. Results: The co-expression of PR and CD146 in the endometrioid adenocarcinoma can be detected by QDs double-labeling immunofluorescence, and there was no correlation between them (P > 0.05). Conclusion: QDs double-labeling immunofluorescence can detect the localization and co-expression of PR and CD146 in the endometrioid adenocarcinoma.

Comparison of indirect immunofluorescence and western blot method in the diagnosis of hantavirus infections

BACKGROUND Serologic cross-reactivity between hantaviruses often complicates the interpretation of the results.AIM To analyze the diagnostic value of indirect immunofluorescence assay(IFA)and western blot(WB)in the diagnosis of hantavirus infections.METHODS One hundred eighty-eight serum samples from Puumala(PUUV)and Dobrava(DOBV)orthohantavirus infected patients were analyzed.Serology was performed using commercial tests(Euroimmun,Lübeck,Germany).RESULTS Using IFA,49.5%of acute-phase samples showed a monotypic response to PUUV,while 50.5% cross-reacted with other hantaviruses.The overall cross-reactivity was higher for immunoglobulin G(IgG)(50.0%)than for immunoglobulin M(IgM)(25.5%).PUUV IgM/IgG antibodies showed low/moderate reactivity with orthohantaviruses Hantaan(12.3%/31.5%),Seoul(7.5%/17.8%),DOBV(5.4%/28.1%),and Saaremaa(4.8%/15.7%).Both DOBV IgM and IgG antibodies were broadly reactive with Hantaan(76.2%/95.2%),Saaremaa(80.9%/83.3%),and Seoul(78.6%/85.7%)and moderate with PUUV(28.5%/38.1%).Using a WB,serotyping was successful in most cross-reactive samples(89.5%).CONCLUSION The presented results indicate that WB is more specific than IFA in the diagnosis of hantavirus infections,confirming serotype in most IFA cross-reactive samples.

New highly specific anti-BnASY polyclonal antibody prepara-tion and application in immunofluorescence assay

ASY （asynaptic） is a synaptonemal complex （SC） related protein in plant mei- osis. Some ASYs in plants have been cloned and functional determined. ASY in Brassica napus has not been sequenced and functional certificated. Here, we first cloned ASY gene in Brassica napus （BnASY） and inserted it into vector pET-32a for expression fusion protein BnASY-6His in Escherichia coli BL21 （DE3）. Purified fusion protein was used to produce polyclonal antibody. Specificity and application of polyclonal antibody was examined by Western blot and immunofluorescence assay. Results showed that BnASY-6His recombi-nant protein and anti-BnASY antibody were successfully obtained. Polyclonal anti-BnASY antibody had high specificity. Results of immunofluorescence showed that ASY signals appeared at leptotene stage, faded away gradually at pachytene stage and almost disap-peared at diplonema stage. In this study, highly specific polyclonal antibody was success-fully acquired and used for immunofluorescence assay in plant cells. It will contribute to functional research of ASY in B. napus.We thank Zhigang Li for providing pET-32a vector and Escherichia coli BL21 pLysS strains.

真菌病毒Beauveria bassiana chrysovirus 2(BbCV2)外壳蛋白多克隆抗体制备及应用

球孢白僵菌Beauveriabassiana是一种在害虫生物防治中应用广泛的虫生真菌,真菌病毒能够影响球孢白僵菌的致病力和生物学性状,但真菌病毒相关蛋白的抗体制备和利用其进行病毒检测和定位鲜有报道。本研究原核表达了一株普遍流行并且造成寄主球孢白僵菌毒力下降的双链RNA(double stranded RNA,dsRNA)病毒Beauveria bassiana chrysovirus 2(Bb CV2)的外壳蛋白(Coat protein,CP),并制备了多克隆抗体,进行了病毒在寄主球孢白僵菌胞内和胞外的检测,以及利用间接免疫荧光进行病毒在寄主内的定位。结果表明,表达的BbCV2-CP蛋白主要以包涵体的形式存在,相对分子质量约为85.7kD;经间接ELISA方法测定,制备的BbCV2-CP兔源多抗效价达到1:8192000;Westernblot结果显示,制备的BbCV2兔源多抗能与抗原蛋白进行特异性结合,且能检测出感染寄主球孢白僵菌的BbCV2;ELISA测定结果表明病毒BbCV2可在寄主真菌体内复制,并能够游离到寄主体外;经间接免疫荧光观察,发现BbCV2病毒定位于真菌细胞核中。本研究建立了球孢白僵菌真菌病毒的血清学检测体系,为球孢白僵菌-真菌病毒互作机制研究提供材料。

果胶酶对灵武长枣果实发育中阿拉伯半乳糖蛋白分布的影响

以3种不同浓度的果胶酶处理灵武长枣(Ziziphus jujuba‘Lingwu Changzao’)4个不同发育时期的果实,采用免疫细胞化学技术,在细胞水平上对果实阿拉伯半乳糖蛋白(AGPs)表位进行原位分析,探讨果胶酶对其不同发育时期的果实中AGPs分布的影响,为明确果胶酶对果实成熟软化的影响提供解剖学依据。结果表明:JIM13、JIM8和MAC204抗体所标记的抗原荧光强弱在各时期果实的不同组织存在一定的差异。当果肉组织用较低浓度的果胶酶0.028 U·mL^(-1)(E1)处理,果皮组织结构没有明显的变化,果皮及内部薄壁细胞细胞壁表面和细胞间隙中的AGPs抗原表位减少;0.056 U·mL^(-1)(E2)和0.084 U·mL^(-1)(E3)浓度果胶酶处理的果实,果实组织细胞壁解体程度增加,果皮及内部薄壁细胞细胞壁中AGPs抗原表位检测量逐渐降低,果胶酶浓度的增加导致AGPs在果实所有表位排列的更大影响和较低的荧光信号。经果胶酶最高浓度0.084 U·mL^(-1)(E3)处理后,Calcofluor White染色显示细胞壁区域荧光也不同程度减弱或降低,AGPs分布的紊乱和抗原表位的缺失与细胞中纤维素组装的变化有关。比较分析表明,不同发育时期的果实AGPs碳水化合物的分布不同,这与组织结构的变化有关;果胶酶作用下AGPs聚糖链的缺失导致细胞壁组分之间的相关性建立和细胞壁结构的重塑受阻,诱导了整个细胞壁结构的改变,影响了果实的成熟。

多重微球流式免疫荧光技术对肺癌患者外周血IL-1β、IL-6、IFN-γ水平测定及与hs-CRP的相关性分析

目的探讨多重微球流式免疫荧光技术在肺癌患者外周血白细胞介素(IL)-1β、IL-6和干扰素γ(IFN-γ)细胞因子的表达情况及与超敏C反应蛋白(hs-CRP)相关性分析。方法采用回顾性研究的方法,选择张家港市中医医院(下称该院)肿瘤科和肺病科收治的30例肺癌患者作为肺癌组,另选择同期该院收治的30例肺炎患者作为肺炎组,同时选取同期该院体检健康者30例作为对照组,通过多重微球流式免疫荧光技术检测血清中IL-1β、IL-6和IFN-γ水平,同时利用乳胶增强免疫散射比浊法测定外周血全血中hs-CRP水平。结果肺癌组与对照组比较,IL-1β、IL-6和hs-CRP水平显著升高,差异有统计学意义(P<0.001),而IFN-γ水平差异无统计学意义(P>0.05);肺炎组与对照组比较,IL-1β、IL-6、IFN-γ、hs-CRP水平均显著升高,差异有统计学意义(P<0.001);肺癌组与肺炎组比较,IL-6、IFN-γ、hs-CRP水平明显降低且IL-1β水平升高,差异均有统计学意义(P<0.05);肺癌组、肺炎组IL-6和hs-CRP水平分别进行Pearson相关性分析,均无明显的相关性。结论IL-1β、IL-6、IFN-γ可以作为有效评估肺癌患者免疫功能的辅助指标,多重微球流式免疫荧光技术的应用对于肺癌的诊断及监测具有潜在的临床应用价值。

鸡马立克氏病火鸡疱疹病毒间接免疫荧光检测方法的建立与比较

为建立鸡马立克氏病火鸡疱疹病毒(MDV HVT)的间接免疫荧光方法,将MDV HVT病毒接种96孔细胞板培养(CEF),72 h后用鸡抗马立克氏病病毒阳性血清作为一抗和兔抗鸡荧光抗体作为二抗,对反应条件进行优化,建立了间接免疫荧光方法(IFA)。并与经典的马立克蚀斑计数方法进行病毒滴度的测定比较,运用统计学方法分析,P小于0.05,相关系数为0.995,说明两种方法相关性很好,两种方法均可用于马立克氏病病毒的滴度测定。IFA方法较蚀斑计数方法操作简便快捷,可代替蚀斑计数方法用于马立克氏病活疫苗的病毒含量的初步测定,同时为2025年版《中国兽药典》马立克氏病活疫苗增加IFA鉴别检验方法积累实验数据。

皮肤石蜡组织Ⅳ型胶原免疫荧光抗原修复方法的评估

目的 寻找皮肤石蜡包埋组织Ⅳ型胶原免疫荧光(IF-PE)最佳抗原修复方法。方法以2021年1月至2022年12月在上海交通大学医学院附属儿童医院确诊的X-连锁Alport综合征患儿和父(母)亲共14例皮肤组织,冰冻组织免疫荧光(IF-FT)为自身对照,比较不同抗原修复法IF-PE染色部位和强度。结果 与Ⅳ型胶原IF-FT自身对照比较,采用蛋白酶K修复,仅部分患儿基膜正常分布(6/14),而角质层均异常表达;微波、高温水浴和高压蒸汽3种修复方法,基膜均无正常分布,角质层异常分布(分别为2/14,11/14,12/14);微波联合酶修复法仅2例基膜正常分布,未见角质层异常表达;高压蒸汽联合酶和高温水浴联合酶2种修复法基膜全部正常分布,角质层异常表达(分别为14/14和2/14),表达强度两者接近。结论高温水浴联合蛋白酶K可作为皮肤石蜡包埋组织Ⅳ型胶原免疫荧光理想的抗原修复法。

当归多糖促进骨髓移植重建受体小鼠造血功能

目的探讨当归多糖(ASP)调控骨髓基质细胞(BMSCs)促进供体骨髓移植(BMT)重建受体小鼠造血功能的机制。方法分离纯化8~10周龄雄性C57BL/6J小鼠骨髓单个核细胞(BMMNCs),移植给同龄同种雌性受体小鼠,第9天取受体鼠BMMNCs,再次移植给雌性受体小鼠。移植受体鼠分为对照组:假照射;辐射组:8.0 Gy X射线全身一次性照射;骨髓移植组:照射同辐射组,经尾静脉移植雄性供体BMMNCs(5×10^(6)个细胞);骨髓移植ASP组:同骨髓移植组,从移植的第1天起连续腹腔注射ASP[100 mg/(kg·d)×9]。模型构建期间记录小鼠体重与生存变化,模型构建结束后采集受体小鼠BMMNCs检测Y染色体性别决定区(SRY)基因,测定外周血血常规指标,计算股骨BMMNCs数,观察骨髓组织病理学;分离培养受体鼠BMSCs,观察细胞贴壁生长,5-乙炔基-2’-脱氧尿苷(EdU)法检测BMSCs增殖;分析细胞内活性氧(ROS)水平、超氧化物歧化酶(SOD)活性及丙二醛(MDA)含量;检测BMSCs培养上清液中粒细胞-巨噬细胞集落刺激因子(GM-CSF)、干细胞因子(SCF)和胰岛素样生长因子1(IGF-1)水平,检测BMMNCs与各组BMSCs共培养48 h,形成造血祖细胞混合集落(CFU-Mix)数量;Real-time PCR分析受体BMMNCs的Notch信号通路相关基因(Notch1、Jagged1、Hes1)表达。结果单纯辐射组小鼠全部死亡,骨髓移植ASP组受体鼠体重下降不明显;在受体雌鼠BMMNCs中检测到SRY基因;骨髓移植ASP组受体鼠外周血血常规和BMMNCs总数下降幅度不显著,骨髓组织病理学损伤减轻;ASP能促进BMSCs增殖,降低BMSCs中ROS、MDA含量,提高SOD活性;促进BMSCs分泌SCF、GM-CSF及IGF-1,提高BMMNCs与受体BMSCs共培养后的CFU-Mix产率;提高受体小鼠BMMNCs中Notch1、Jagged1、Hes1 mRNA表达。结论ASP促进受体小鼠造血功能重建机制与减轻造血微环境氧化应激损伤,提高BMSCs分泌造血生长因子,调控Notch信号通路有关。

不同途径感染禽网状内皮组织增殖病病毒的动态监测

为明确鸡群经不同途径感染禽网状内皮组织增殖病病毒(REV)的排毒动态,本试验通过设立无特定病原体(SPF)鸡胚6胚龄卵黄囊感染组、1日龄SPF鸡腹腔感染组以及对上述两组SPF鸡分别加入感染鸡的卵黄囊感染同居组和腹腔感染同居组,建立SPF鸡感染REV模型,同时设置空白对照组,在不同日龄记录各组鸡的体重和死亡情况,并综合运用反转录PCR(RT-PCR)、实时荧光定量PCR(RT-qPCR)和间接免疫荧光试验(IFA)3种检测方法对各感染组进行REV的动态监测。结果显示:(1)与空白对照组相比,腹腔感染组和卵黄囊感染组SPF鸡体重增长在感染后第21~70天均受到显著抑制(P<0.05),卵黄囊感染组SPF鸡的死亡率在感染后第49和63天显著升高(P<0.05),腹腔感染组SPF鸡的死亡率在感染后第42天显著升高(P<0.05),卵黄囊感染组SPF鸡血浆中REV病毒载量在感染后第21天显著高于腹腔感染组(P<0.05);(2)卵黄囊感染组SPF鸡自出壳即可检测到病毒血症阳性,并在感染后第21天时达到排毒高峰,腹腔感染组SPF鸡在感染后第14天时达到排毒高峰;(3)卵黄囊感染同居组的10只SPF鸡在感染后第7天时即检测到2只鸡呈病毒血症阳性,腹腔感染同居组SPF鸡在感染后第21天时检测到1只鸡呈阳性;(4)3种检测方法中,RT-qPCR和IFA检出REV效果更好。本试验通过分析不同途径感染REV后鸡群血浆中的带毒状态,为REV感染的科学防控和净化提供参考数据。

毒害艾美耳球虫谷胱甘肽过氧化物酶EnGPX的原核表达与分析

旨在研究毒害艾美耳球虫谷胱甘肽过氧化物酶EnGPX的反应原性及其在虫体内的亚细胞定位。提取毒害艾美耳球虫(扬州株)配子体总RNA,RT-PCR扩增En GPX的ORF编码序列,构建原核表达质粒pET-28a(+)-En GPX,转化至BL21(DE3)进行体外诱导表达,同时制备鼠抗rEnGPX多克隆抗体,对重组蛋白进行Western blot反应原性分析和激光共聚焦免疫荧光定位分析。结果表明,En GPX ORF序列全长753 bp,编码250个氨基酸,体外重组表达蛋白大小约30 ku,主要以包涵体形式存在。该重组蛋白能被6×HIS标签单克隆抗体,鼠抗rEnGPX多克隆抗体,毒害艾美耳球虫、巨型艾美耳球虫和柔嫩艾美耳球虫病鸡康复血清所识别,表明其具有较好的反应原性和交叉反应原性。在天然配子体蛋白中检测出EnGPX,其编码蛋白主要分布于配子体内的Ⅱ型成壁体(WFBII)及卵囊壁上。本研究成功克隆表达了毒害艾美耳球虫谷胱甘肽过氧化物酶EnGPX,验证其具有良好的反应原性,并定位于配子体及卵囊壁上。以期为研究En GPX参与卵囊壁形成的分子机制提供新的线索,也为研制新型球虫亚单位疫苗提供新的靶标。

免疫荧光技术在近视相关生物标志物检测中的应用进展

免疫荧光(IF)技术亦称荧光抗体技术,是通过结合荧光团标记的特定抗原或抗体在紫外线发出荧光来实现的一种示踪技术。IF具有极高的灵敏度和信号放大能力,被广泛应用于细菌病毒和寄生虫的鉴别诊断、部分疾病免疫学机制的研究、器官移植的鉴定、抗原组织定位等方面。近视作为一种屈光不正性疾病,严重影响着人们的视力健康,IF在近视机制及治疗措施的研究中发挥了重要作用。本文就近年来IF在近视相关生物标志物检测中的应用进展进行综述。

免疫荧光检测石蜡切片IgA蛋白在诊断疱疹样皮炎和线状IgA大疱性皮病的应用评价

目的:评价直接免疫荧光染色检测石蜡切片IgA抗体对于诊断疱疹样皮炎(DH)和线状IgA大疱性皮病(LABD)的应用价值。方法:选取2019-2024年我院病理诊断的DH和LABD病例,入选实验组病例DH 46例,LABD 32例。采用FITC荧光标记兔抗人IgA抗体进行直接免疫荧光染色检测。结果:46例DH石蜡切片中,40例IgA在真皮乳头为阳性,阳性率86.96%。32例LABD石蜡切片中,20例IgA在表皮基底膜线状沉积为阳性,阳性率62.50%。结论:直接免疫荧光染色检测石蜡切片IgA可以作为辅助诊断DH和LABD的有效方法。

直接免疫荧光技术联合组织病理及血清抗体检测应用于黏膜类天疱疮的诊断准确性探究

目的探讨在组织病理学及血清特异性抗体检测基础上,联合直接免疫荧光技术(DIF)对黏膜类天疱疮(MMP)诊断效能的影响。方法纳入MMP患者29例,对照组29例,切取活检组织分别进行苏木精-伊红(HE)及DIF染色,对仅使用组织病理学及血清特异性抗体检测,和联合使用DIF后两种诊断方法进行诊断效能评价,分析多种因素对组织病理学及DIF诊断准确性的影响。结果联合使用DIF后可以提高MMP的诊断敏感度、阴性预测值、诊断符合率和受试者操作特征(ROC)曲线下面积。病程长短对DIF诊断准确性有显著影响,病程越长,DIF诊断准确性越高(P<0.05)。结论DIF联合组织病理学及血清抗体检测可以提高MMP的诊断准确性。对于疑难病例可能需要通过多次、多部位的活检提高DIF对MMP的诊断率。

用于多重免疫荧光染色的小鼠肺组织冰冻切片制备方法优化研究

目的优化小鼠肺组织冰冻切片制作方法,提高肺组织冰冻切片质量,有利于提高免疫荧光染色的特异性,获得更准确可靠的实验结果。方法使用C57BL/6小鼠,分别采用传统冷冻后固定法、冷冻前固定法、改良灌注冷冻前固定法3种方法制作冰冻切片,经免疫荧光染色后使用激光扫描共聚焦荧光显微镜观察肺组织染色情况。使用荧光显微镜对肺组织切片进行全片扫描,计算单位面积内完整气道数量。结果传统冷冻后固定法制作的小鼠肺组织冰冻切片,肺泡结构破坏,气道壁断裂严重,存在非特异性染色;冷冻前固定法制作的小鼠肺组织切片,肺泡和气道结构相对完整,但肺泡塌陷,部分气道结构破坏;改良灌注冷冻前固定法制作的小鼠肺组织切片,肺泡和气道结构形态均完整、清晰,多重免疫荧光染色定位准确。改良灌注冷冻前固定法制作的小鼠肺组织冰冻切片单位面积内完整气道(直径≥100μm)数量高于冷冻前固定法((0.66±0.15)/mm^(2) vs(0.33±0.14)/mm^(2),P<0.05),也显著高于传统冷冻后固定法((0.66±0.15)/mm^(2) vs(0.02±0.04)/mm^(2),P<0.01)。结论使用改良灌注冷冻前固定法制作冰冻切片,利于保持小鼠肺组织形态完整,利于获得高质量的多重免疫荧光染色结果。

南京地区健康人群血清可溶性程序性死亡蛋白-1参考区间的建立

目的探讨健康人群血清可溶性程序性死亡蛋白-1(soluble programmed cell death protein-1,sPD-1)水平及其影响因素,初步建立南京地区健康人群血清sPD-1水平的参考区间。方法本研究纳入2023年5月至9月在南京鼓楼医院及句容人民医院进行体检的健康人群375例,其中男性194例,女性181例。留取健康人群的血清标本,采用基于新型探针生物传感器的全自动荧光免疫分析法(tests-on-probes,TOP法)检测血清sPD-1水平,并分析性别、年龄及其他实验室指标对sPD-1的影响;采用非参数法计算总体及不同年龄段健康人群血清sPD-1水平的参考区间。结果健康人群血清sPD-1水平为108.82(92.80,134.95)pg/mL,男性和女性健康人群血清sPD-1水平差异无统计学意义(P>0.05)。进一步将健康人群按照年龄分为<65岁和≥65岁2组,其血清sPD-1水平分别为106.65(90.35,130.60)pg/mL,113.20(95.60,144.83)pg/mL,组间差异有统计学意义(P=0.014);而将健康人群根据年龄分成3组(<40岁,40~64岁,≥65岁)时,其血清sPD-1水平分别为112.00(98.68,137.23)pg/mL,99.07(82.38,119.60)pg/mL,113.20(95.60,144.83)pg/mL,3组间差异亦有统计学意义(P<0.001)。多因素线性回归分析显示,γ-谷氨酰基转移酶(γ-glutamyl transpeptidase,GGT)是健康人群血清sPD-1水平的影响因素。根据临床与实验室标准协会(Clinical and Laboratory Standards Institutes,CLSI)C28-A3文件推荐的非参数法计算sPD-1参考区间,健康人群总体血清sPD-1水平的参考区间(第2.5%~97.5%百分位的浓度范围)为66.7~214.7 pg/mL;将健康人群分为<40岁、40~64岁、≥65岁3个年龄段,其对应的血清sPD-1在第2.5%~97.5%百分位的浓度范围分别为71.9~202.7 pg/mL、59.4~220.0 pg/mL、69.6~229.0 pg/mL。结论本研究初步建立了南京地区血清sPD-1健康人群以及分为3个年龄段的参考区间。