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.

Detection of Atrazine Residue in Food Samples by a Monoclonal Antibody-based Enzyme-linked Immunosorbent Assay

Atrazine（AT,2-chloro-4-ethylamino-6-isopropyl-amino-s-triazine）has been detected in ground water in several areas of the United States for many years,as well as in China,wherein the growth rate of its gross

Quantitative determination of erlotinib in human serum using competitive enzyme-linked immunosorbent assay

A selective and sensitive competitive enzyme-linked immunosorbent assay(ELISA) method was developed and validated for the quantification of erlotinib in 50 mL of samples of human serum. Anti-erlotinib serum was obtained by immunizing mice with an antigen conjugated with bovine serum albumin and 3,4-bis(2-methoxyethoxy)benzoic acid using the N-succinimidyl ester method. Enzyme labeling of erlotinib with horseradish peroxidase was similarly performed using 3,4-bis(2-methoxyethoxy)benzoic acid. A simple competitive ELISA for erlotinib was developed using the principle of direct competition between erlotinib and the enzyme marker for anti-erlotinib antibody, which had been immobilized on the plastic surface of a microtiter plate. Serum erlotinib concentrations lower than 40 ng/mL were reproducibly measurable using the ELISA. This ELISA was specific to erlotinib and showed very slight cross-reactivity(6.7%) with a major metabolite, O-desmethyl erlotinib. Using this assay, drug levels were easily measured in the blood of mice after oral administration of erlotinib at a single dose of 30 mg/kg. ELISA should be used as a valuable tool for therapeutic drug monitoring and in pharmacokinetic studies of erlotinib.

Development of a competitive enzyme-linked immunosorbent assay for therapeutic drug monitoring of afatinib

Afatinib is an oral tyrosine kinase inhibitor(TKI) approved for treating advanced non-small cell lung cancer. It is necessary to develop a simple quantification method for TKIs in order to facilitate therapeutic drug monitoring(TDM) in clinical settings. This study sought to develop a simple and sensitive competitive enzyme-linked immunosorbent assay(ELISA) to quantify afatinib in plasma for routine pharmacokinetic applications. An anti-afatinib antibody was obtained using(S)-N-4-(3-chloro-4-fluorophenyl)-7-(tetrahydrofuran-3-yloxy)-quinazoline-4,6-diamine(CTQD), which has the same substructure as afatinib, as a hapten. Enzyme labeling of afatinib with horseradish peroxidase was similarly performed using CTQD. A simple competitive ELISA for afatinib was developed based on the principle of direct competition between afatinib and the enzyme marker for the anti-afatinib antibody, which had been immobilized on the plastic surface of a microtiter plate. Plasma afatinib concentrations below the limit of quantification of 30 pg/mL were reproducibly measurable. Also, the values of plasma afatinib levels measured from 20 patients were comparable with those measured by high-performance liquid chromatography, and there was a strong correlation between the values determined by both methods(Y=0.976 X – 0.207, r=0.975). As indicated by its specificity and sensitivity, this newly developed ELISA for afatinib is an important tool for TDM and studies of the pharmacokinetics of afatinib.

Enzyme-linked Immunosorbent Assay for Detection of Anti-idiotype Antibodies to Antibodies to Ligand of Nicotinic Acetylcholine Receptor in Sera of Patients with Myasthenia Gravis

Anti-bungarotoxin anti-serum,which has the internal image of nicotinicacetylcholine receptor,was used as a tool to measure anti-idiotypic antibodies toantibodies to Iigand of nicotinic acctylcholine receptor in scra from 81 patients withmyasthenia gravis.Enzyme-linked immunosorbcnt assay was adopted.Thc positive ratewas 46.9%(38/81).The specific cross inhibitory test with nicotinic acetylcholinereceptor was positive.Anti-idiotype antibodies to antibodies to ligand of nicotinicacetylcholine receptor in sera of different types of myasthenia gravis patients classified ac-cording to modified Osserman’s standard and myasthenia gravis patients with or withoutthymoma were comparcd in this study and the role of anti-idiotype antibodies toantibodies to Iigand of nicotinic acctylcholinc receptor in the immunity of myasthcniagravis and the possibility of thcrapeutic use of anti-idiotype antibodies arc discussed.

Development of an Indirect Enzyme-Linked Immunosorbent Assay for Seromonitoring Contagious Bovine Pleuropneumonia Using Recombinant Lipoprotein LppQ of Mycoplasma mycoides subsp mycoides SC as Antigen

Mycoplasma mycoides subsp mycoides SC （MmmSC） is the etiological agent of contagious bovine pleuropneumonia （CBPP）. The lipoprotein LppQ encoded by lppQ gene is specific to MmmSC and is found in the type strain and in field strains isolated in Europe, Africa, and Australia, as well as in vaccine strains. No serological cross-reactions were observed with the related mycoplasmas of the Mycoplasma mycoides cluster. The N-terminal domain of the mature lipoprotein LppQ is hydrophilic, and it induces a strong, specific, early, and persistent immune response in naturally and experimentally infected animals. Mycoplasma-specific TGA （Trp） codons are utilized as stop codons in most other organisms. The lppQ N-terminal fragment from MmmSC HVRI X strain, the Chinese strain for CF antigen production, was mutated with one-step overlapping extension PCR. Sequence analysis confirmed the successful mutation from A to G in codon 198 in the lppQ gene. The fragment containing the mutation site was subcloned into the pET32a expression vector. The recombinant protein with molecular weight of 42 kDa was purified using the Ni-NTA His.Bind purification kit, with a purity of up to 95%. Western blot indicated that the standard positive serum of CBPP could react with the recombinant protein. The purified protein was diluted to 0.35 μg mL^-1, and coated to microtiter enzyme-linked immunosorbent assay （ELISA） plates. Indirect ELISA reaction conditions were optimized. The value of P/N was determined to be 4.8 （0.934/0.193）, the sensitivity to be 95.8% （46/48）, and the specificity to be 98.9% （161/163）. 3 817 cattle serum samples from three different provinces were detected by the indirect ELISA and CFT. The Kappa value is 0.63, which is middle or high agreement between the two methods.

A Comparison of Enzyme-Linked Immunosorbent Assay versus Multiplex Methodology Using an <i>in Vitro</i>Model of Pulmonary Hypertension and Inflammation

Enzyme-linked immunosorbent assay (ELISA) is the most widely used method for measuring a single cytokine. Recent developments in cytokine quantification such as multiple arrays measure multiple cytokines simultaneously. Although good correlations between ELISA and multiplex methods have been observed, side by side comparisons are limited. In the present study we hypothesized that ELISA and Luminex techniques are comparable in detecting cytokines in culture medium when pulmonary artery smooth muscle cells (PASMC) are exposed to stress. Primary human PASMC were cultured in modular chambers and exposed to 21% FiO2 and peak inspiratory and positive end expiratory pressure of 24 and 8 cmH2O respectively, and 95% FiO2. At 24 hours, culture medium was collected and assayed for interleukin-6 (IL-6) and IL-8 by quantitative ELISA and by Human Cytokine 25-Plex Panel using a Luminex 200 analyzer. A comparative analysis of agreement between our ELISA and Luminex data was detailed for control and stress conditions using the Bland-Altman plot analysis. Each assay resulted in comparable increased (p < 0.001) levels of IL-6 and IL-8 as compared to control in response to oxidative and biophysical stress. The Bland-Altman analysis demonstrated that 95% of the differences between ELISA and Luminex values were within ±1.96 SD from the mean difference indicated by the 95% limits of agreement for the measurements of IL-6 and IL-8. There was no systematic bias as a function of inflammation level. We conclude that in this cell culture model, ELISA and Luminex are comparable in detecting the levels of IL-6 and IL-8 in the culture medium. If measurements of multiple cytokines are demanded and the amount of sample is limited, Luminex multi-analyte profiling technology is accurate and sensitive.

ENZYME-LINKED IMMUNOSORBENT ASSAY OF HUMAN PLACENTA TYPE GLUTATHIONE S-TRANSFERASE AND ITS APPLICATION IN THE DIAGNOSIS OF HEPATOCARCINOMA

GST-π was purified from human placenta and its antiserum was raised in rabbits. The antibody IgC was purified and degraded into Fab' fragment which was conjugated with horseradish peroxidase (HRP) using N-succinimidyl-4-(N-maleimido-methyl) cyclo-hexane-1-carboxylate (SMCC) as crosslinking reagent to produce Fab'-HRP conjugate. A sandwich ELISA was established for the microquantitative determination of GST-π. The sensitivity was 11 pg/tube, which was far more sensitive than the radioimmunoassay so far reported. Using this method, the serum GST-π of 41 cases normal adult was found to be 1.06±0.94 ng/ml. The upper limit of the normal value was 2.6 ng/ml. In 30 cases of primary hepatocarcinoma, the level of serum GST-π was 24.4± 17.4 ng/ml, which was 23 times higher than the normal average value (P<0.01). The positive rate was 90%. In contrast, serum GST-π in 25 cases of chronic hepatitis was determined to be 1.74±1.16 ng/ml, which was not significantly different from the normal value (P>0.05). The pseudo-positive rate was 12.0%.

Determnation of ochratoxin A in grain by monoclonal antibody－based enzyme－linked immunosorbent assay

The simple rapid and sensitive enzyme-linked immunosorbent assay (ELISA) methods, di-rect and indirect ELISA, for quantitation of ochratoxin A in cereal had been developed by theutilization of monoclonal antibody on immunomicroplate. Direct FLIAS was found to be less timeconsuming than indirect ELISA. For direct FLISA, recovery of 1 -500 ppb OA added to wheat was78.9-100.0% and rice was 88.9- 120.0%. For indirect EI.IAS, recovery of 1-500 ppb OA addedto wheat was 79.0- 110.0% and rice was 82.0 120.0%. The minimal detection level for OA was Ippb. Analyses of 31 samples that caused humanintoxicant for OA showed that the ELISA resultsagreed wtll with those obtained by thin-layer chromatogrdphy.

免疫亲和层析技术协同酶联免疫吸附法检测赭曲霉毒素A

利用免疫亲和层析技术(immunoaffinity chromatography,IAC)对样品中赭曲霉毒素A(ochratoxin A,OTA)进行捕获与浓缩,利用酶联免疫吸附(enzyme-linked immunosorbent assay,ELISA)法对IAC捕获的目标物OTA进行测定。IAC与ELISA中的抗OTA单克隆抗体来自不同的克隆株,分属不同独特型,与OTA结合靶点的选择性存在差异,IAC与ELISA协同检测,可以有效过滤OTA结构类似物造成的干扰,提高免疫分析的特异性与灵敏度。该方法用于加标样品测定时,OTA的检出限为0.2 ng/g,定量限为0.4 ng/g,OTA的平均回收率为75.9%,与单一的ELISA法相比,该方法虽然回收率略低,但灵敏度可以显著提高,达到ELISA法的60倍。通过对49份样品的实际检测,该方法检出阳性样品与国标法的符合率达到100%,漏检率为0%,由此可见,该方法在准确性上表现出明显的优势。作为一种综合免疫分析技术,该方法不需要大型仪器设备,对操作环境没有严格要求,便于基层实验室对样品中OTA的分析。

综合洗消体系对阻断非洲猪瘟病毒传入猪场的作用

切断非洲猪瘟病毒(ASFV)传播途径是防控非洲猪瘟的有效手段。本试验旨在通过在某种猪场建立综合洗消体系以阻断ASFV传入。对拟进入猪场的车辆在出发前和距猪场1 km处清洗和消毒,在猪场门口进行第3次消毒;人员进入猪场前洗澡和隔离,并将其衣物消毒;输入物资进场前消毒。通过实时荧光定量PCR检测经洗消的车辆、人员、物资和猪场内猪只携带ASFV核酸情况,酶联免疫吸附测定(ELISA)检测猪只的ASFV抗体水平。结果显示,2019、2020、2021和2022年,车辆ASFV检出率分别为2.6%、1.3%、0和0,人员ASFV检出率分别为3.0%、1.1%、0和0.9%,物资ASFV检出率分别为12.5%、0、5.9%和0;4年间,猪场内猪只的ASFV核酸和抗体检测均为阴性。结果表明,通过建立完善的洗消体系并开展ASFV检测,能有效阻断ASFV传入猪场。

基于化学发光酶免疫分析法检测花生过敏原Ara h 2

Ara h 2是花生主要过敏原之一,为开发食物中Ara h 2过敏原成分的快速检测方法,减少因误食导致花生过敏事件的发生,该研究采用鼠源单克隆抗体作为捕获抗体、兔源多克隆抗体作为检测抗体,通过棋盘法优化抗体工作浓度,建立了一种检测花生过敏原Ara h 2的间接双抗夹心化学发光酶免疫分析法,并对该方法的灵敏度、准确度、精密度和特异性进行评价。该方法的检出限为1.085 ng/mL,线性范围为3.12~200 ng/mL,添加回收率为78.30%~94.39%,批内和批间变异系数均小于10%,且特异性良好,与其他常见食物过敏原无交叉反应。该方法与相同抗体所建立的间接双抗夹心酶联免疫吸附测定(enzyme-linked immunosorbent assay, ELISA)方法相比,在灵敏度上表现出一定优势。该研究开发的化学发光酶免疫分析法可对花生食品生产过程中和消费前的Ara h 2过敏原成分检测提供可靠的技术支持。

2016至2020年杭州地区无偿献血人群HIV感染状况分析

目的了解杭州地区无偿献血人群HIV感染状况,为本地区降低HIV经输血传播风险,制定有效献血者招募及艾滋病防控策略提供数据支持。方法采用酶联免疫吸附试验(enzyme-linked immunosorbent assay,ELISA)和病原体核酸检测技术(nucleic acid testing,NAT)对2016年1月至2020年12月杭州地区902847例无偿献血者标本进行抗HIV-Ⅰ/Ⅱ抗体/抗原和HIVRNA检测。抗-HIV抗体/抗原或HIVRNA反应性标本送杭州市疾病控制中心进一步采用Western blot法和NAT进行确认。结果2016年1月至2020年12月杭州地区共检测HIV确证阳性103例,阳性检出率为0.01%,其中101例ELISA和NAT筛查均为阳性反应,2例ELISA筛查为阴性反应,NAT为阳性反应。103例感染者中,以男性(91.26%,94/103)、18~35岁(69.90%,72/103)、初次献血者(68.93%,71/103)为主。2016至2020年献血者HIV阳性率呈逐年下降趋势(χ^(2)=7.181,P=0.007)。男女献血者HIV阳性率各年的差异无统计学意义(χ^(2)=10.336,P=0.350;χ^(2)=0.653,P=0.957)。各年龄组献血者HIV阳性率各年的差异无统计学意义(χ^(2)=6.378,P=0.173;χ^(2)=2.318,P=0.678;χ^(2)=5.284,P=0.259;χ^(2)=9.183,P=0.057)。结论近5年HIV感染在杭州市无偿献血人群中呈低流行水平,但仍存在感染风险,应加强在低危人群中招募献血者并且应采用先进的检测技术,选择合适的检测策略,保证血液安全。

两种不同免疫检验方法检测乙型肝炎病毒感染血清学标志物的临床疗效

目的分析两种不同免疫检验方法检测乙型肝炎病毒感染血清学标志物的临床疗效。方法回顾性分析2021年6月至2022年6月枣庄市立医院收治的88例乙型肝炎患者的临床资料,所有患者均确诊为乙型肝炎病毒感染,并采用磁微粒化学发光法、酶联免疫吸附法检测乙型肝炎病毒感染血清学标志物。比较两种免疫检测方法对乙型肝炎病毒感染血清学标志物的检出情况和诊断准确率。结果磁微粒化学发光法对乙型肝炎病毒表面抗原、乙型肝炎病毒e抗原、乙型肝炎病毒e抗体的阳性检出率高于酶联免疫吸附法,差异有统计学意义(P<0.05);两种免疫检验方法对乙型肝炎病毒表面抗体、乙型肝炎病毒核心抗体的阳性检出率比较差异无统计学意义。磁微粒化学发光法对乙型肝炎表面抗原浓度≤0.50 IU/ml的检出率高于酶联免疫吸附法,差异有统计学意义(P<0.05)。磁微粒化学发光法对乙型肝炎病毒感染诊断准确率高于酶联免疫吸附法,差异有统计学意义(P<0.05)。结论采用电化学发光法可提高乙型肝炎病毒血清学标志物的检验准确率,为临床筛查乙型肝炎病毒感染提供有力支持。

免疫斑点印迹法检测水解乳蛋白婴幼儿配方粉免疫反应

目的:建立一种快速且精准的方法,以确定水解乳蛋白婴幼儿配方粉的免疫反应性。方法:首先采用直接免疫斑点印迹法,利用牛奶过敏患儿血清初步评估待测样品的免疫反应性;然后通过间接竞争免疫斑点印迹法以市售普通牛奶粉为阳性对照,评估水解乳蛋白婴幼儿配方粉与血清免疫球蛋白E(IgE)的结合能力;最后采用间接和间接竞争酶联免疫检测法,以佐证免疫斑点印迹结果。结果:部分水解乳蛋白婴配粉仍可以结合IgE以诱发过敏反应,而深度水解乳蛋白婴配粉不具有免疫反应性。免疫斑点印迹和酶联免疫检测评价免疫反应性结果显著且一致。结论:免疫斑点印迹技术操作性强,周期短,成本低,结果可靠,为利用较难获取的婴幼儿过敏患儿血清初步评估乳蛋白产品致敏性提供了新思路。

急性胆囊炎患者胆囊切除术后血清CCK-8、TREM1水平与发生感染的关系

目的分析急性胆囊炎(AC)患者胆囊切除术后血清胆囊收缩素-8(CCK-8)、髓系细胞触发受体1(TREM1)水平与发生感染的关系。方法将该院2020年12月至2022年12月收治的70例胆囊切除术后发生感染的AC患者纳入研究组,66例胆囊切除术后未发生感染的AC患者纳入对照组。采用酶联免疫吸附试验检测血清CCK-8、TREM1水平。采用Pearson相关分析胆囊切除术后发生感染AC患者血清中CCK-8、TREM1水平与炎症因子水平的相关性。采用受试者工作特征(ROC)曲线分析血清CCK-8、TREM1水平对AC患者胆囊切除术后发生感染的诊断价值。采用多因素Logistic回归分析AC患者胆囊切除术后感染的影响因素。结果研究组与对照组有胆囊结石、胆囊周边积液比例比较,差异均有统计学意义(P<0.05)。与对照组比较,研究组血清CCK-8水平明显降低,TREM1水平明显升高,差异均有统计学意义(P<0.05)。研究组C反应蛋白(CRP)、白细胞介素-8(IL-8)、肿瘤坏死因子-α(TNF-α)水平明显高于对照组,差异均有统计学意义(P<0.05)。胆囊切除术后发生感染的AC患者血清CCK-8水平与CRP、IL-8、TNF-α水平均呈负相关(P<0.05),TREM1水平与CRP、IL-8、TNF-α水平均呈正相关(P<0.05)。ROC曲线分析显示,血清CCK-8与TREM1联合检测诊断AC患者胆囊切除术后发生感染的曲线下面积(AUC)明显大于CCK-8、TREM1单独检测的AUC(Z=5.703,P<0.001;Z=4.584,P<0.001)。有胆囊结石、胆囊周边积液及血清CCK-8水平降低、血清TREM1水平升高均为AC患者胆囊切除术后发生感染的危险因素(P<0.05)。结论胆囊切除术后发生感染的AC患者血清CCK-8水平降低,TREM1水平升高,二者联合检测能够提高对AC患者胆囊切除术后发生感染的诊断价值。

人参联合咖啡因对大鼠的抗疲劳作用及机制探讨

目的评估人参联合咖啡因对大鼠的抗疲劳作用及机制。方法将SD大鼠随机分为空白组、模型组、人参组(60 mg·kg^(-1))、咖啡因组(3.0 mg·kg^(-1))、配伍组(30 mg·kg^(-1)+1.5mg·kg^(-1)),建立大鼠负重游泳疲劳模型,每日给药1次,连续给药21 d;采用负重游泳实验评价药物抗疲劳作用;采用两成分组合效应系数(two components combination index,TCCI)方法评估人参配伍咖啡因抗疲劳协同增效作用;比色法检测各组大鼠的尿素氮(BUN)、乳酸(LD)和肝/肌糖原水平;酶联免疫吸附法检测各组大鼠白细胞介素6(IL-6)、白细胞介素1β(IL-1β)和C反应蛋白(CRP)水平;使用网络药理学初步探讨人参联合咖啡因抗疲劳的可能作用机制。结果人参联合咖啡因TCCI值在0.17~0.61,两者联用显示明显的协同增效作用;与模型组相比,各给药组可不同程度地延长大鼠负重游泳时间,提高肝脏/骨骼肌组织中糖原含量,下调血清中尿素氮水平,降低炎症因子水平;通过网络药理学分析发现,其主要通过PI3K-Akt和MAPK等通路发挥抗疲劳功效。结论人参联合咖啡因可显著降低糖原分解和乳酸等代谢物积累,改善模型大鼠的疲劳症状。

莫米松糠酸酯高特异性抗体制备及酶联免疫分析方法

莫米松糠酸酯(mometasone furoate,MF)是一种常见的糖皮质激素。为快速、便捷地监控MF的滥用情况,制备了MF单克隆抗体并建立了其竞争酶联免疫检测方法。将氨氧乙酸分别连接至MF和莫米松二糠酸酯(mometasone difuroate,MDF),合成了免疫半抗原和包被半抗原。免疫半抗原以活泼脂法连接钥孔血蓝蛋白获得全抗原,通过免疫小鼠、细胞融合及筛选获得能够稳定分泌抗MF单克隆抗体的细胞株,制备并纯化了抗体。该抗体的主要识别区域为MF的五元环区域,因此不和常见的64种糖皮质激素发生交叉反应。建立了基于异源包被的MF间接竞争酶联免疫检测法,其半抑制浓度(IC_(50))为1.2 ng/mL,对肌肉和肝脏的最低检出限分别为0.52μg/kg和0.59μg/kg。灵敏度相比于同源包被提升了20倍。使用60%甲醇水溶液提取动物组织的添加回收率为70%~82%。该方法能有效应用于动物组织中MF的快速筛查。

S-烯丙基巯基半胱氨酸促进CD8+T细胞杀伤功能的机制研究

目的探究S-烯丙基巯基半胱氨酸(S-allylmercaptocysteine,SAMC)对CD8^(+)T细胞杀伤鼻咽癌细胞功能的影响及机制。方法将人鼻咽癌细胞HK-1和C666-1与SAMC共培养,分为0、25、50、100μmol/L SAMC组,Western blot检测肿瘤细胞程序性死亡配体-1(programmed cell death-ligand 1,PD-L1)表达。CD8^(+)T细胞分别与HK-1和C666-1细胞以10∶1的比例共培养并加入0、25、50、100μmol/L SAMC,检测CD8^(+)T对HK-1和C666-1的杀伤能力,酶联免疫法(ELISA)检测干扰素(INF-γ)和肿瘤坏死因子-α(TNF-α)浓度,构建鼻咽细胞HK-1的小鼠皮下移植瘤模型,分为对照组、CD8^(+)T细胞组、SAMC组、SAMC+CD8^(+)T细胞组,各组小鼠治疗期间测量瘤体积,治疗结束后取小鼠肿瘤组织,Western blot检测肿瘤组织中PD-L1表达,ELISA检测小鼠血清INF-γ和TNF-α浓度。结果相比于0μmol/L SAMC组,25、50、100μmol/L SAMC组HK-1和C666-1细胞PD-L1表达均显著下调(P<0.05),相比于0μmol/L SAMC+CD8^(+)T细胞组,25、50、100μmol/L SAMC+CD8^(+)T细胞组HK-1和C666-1细胞培养上清中INF-γ和TNF-α浓度均能显著增加,HK-1和C666-1细胞裂解率显著增加(P<0.01)。相比于对照组,CD8^(+)T细胞组和SAMC+CD8^(+)T细胞组小鼠瘤体积和瘤重显著下降(P<0.05),小鼠血清INF-γ和TNF-α浓度显著增加,相比于CD8^(+)T细胞组,SAMC+CD8^(+)T细胞组小鼠瘤体积和瘤重显著下降(P<0.05),小鼠血清INF-γ和TNF-α浓度显著增加(P<0.05),肿瘤组织PD-L1表达显著下调(P<0.01)。结论SAMC可通过抑制人鼻咽癌细胞PD-L1表达而促进CD8^(+)T细胞的杀伤功能。

酶联免疫吸附法在食品中重金属残留检测中的应用

酶联免疫吸附法(Enzyme Linked Immunosorbent Assay,ELISA)以其高特异性、高灵敏度等优势,在食品重金属残留检测领域展现出广阔的应用前景。本文综述了ELISA检测水产品中汞、谷物中镉、蔬菜中铅、奶制品中铬和食用油中砷的研究进展,重点阐述了抗原设计、抗体制备、样品前处理和检测条件优化等关键技术。针对不同食品基质,提出了进一步提升ELISA检测性能的建议,为食源性重金属分析提供参考。