Miller fisher syndrome with positive anti-GQ1b/GT1a antibodies associated with COVID-19 infection:A case report

BACKGROUND Miller fisher syndrome(MFS)is a variant of Guillain-Barrésyndrome,an acute immune-mediated peripheral neuropathy that is often secondary to viral infections.Anti-ganglioside antibodies play crucial roles in the development of MFS.The positive rate of ganglioside antibodies is exceptionally high in MFS patients,particularly for anti-GQ1b antibodies.However,the presence of other ganglioside antibodies does not exclude MFS.CASE SUMMARY We present a 56-year-old female patient who suddenly developed right blepharoptosis and progressively worsening vision in both eyes.There were flu symptoms prior to onset,and a coronavirus disease 2019 test was positive.On physical examination,the patient exhibited bilateral extraocular muscle paralysis,weakened reflexes in both limbs,and impaired coordination.The cerebrospinal fluid examination results showed no obvious abnormalities.Bilateral peroneal nerve F-waves were not extracted.Serum anti-GD1b IgG and anti-GT1a IgG antibodies were positive.The patient received intravenous methylprednisolone(1000 mg/day),with the dosage gradually decreased.Additionally,intravenous high-dose immunoglobulin treatment was administered for 5 days(0.4 g/kg/day)from day 2 to day 6 of hospitalization.The patient’s symptoms improved after treatment with immunoglobulins and hormones.CONCLUSION Positive ganglioside antibodies may be used as supporting evidence for the diagnosis;however,the diagnosis of MFS is more reliant on clinical symptoms.

Atypical Guillain-Barrésyndrome with positive anti-sulfatide,anti-GT1b,and anti-GT1a antibodies:A case report

BACKGROUND The role of diverse antibodies in mediating peripheral nerve injury in Guillain-Barrésyndrome(GBS)is becoming clearer,but positivity for multiple antibodies in one case is uncommon.To our knowledge,this is the first case involving GBS with positive anti-sulfatide,anti-GT1a,and anti-GT1b antibodies.CASE SUMMARY A 20-year-old female patient was admitted to the hospital due to weakness of limbs for 5 d,and deterioration of the weakness and muscle aches for 1 d.The patient's limbs were weak,but the tendon reflexes in the part of the limbs were normal.There was no comorbid peripheral nociception or deep sensory dysfunction.She was diagnosed with GBS and was discharged after receiving intravenous human immunoglobulin pulse therapy.CONCLUSION In this article,the clinical manifestations,neurophysiological examination,and auxiliary examination findings of a GBS patient positive for multiple antibodies were analyzed to improve the identification of the disease by clinical physicians at an early stage.

Three amino acid residues in the envelope of human immunodeficiency virus type 1 CRF07_BC regulate viral neutralization susceptibility to the human monoclonal neutralizing antibody IgG1b12

The CD4 binding site(CD4bs) of envelope glycoprotein(Env) is an important conserved target for anti-human immunodeficiency virus type 1(HIV-1) neutralizing antibodies. Neutralizing monoclonal antibodies IgG1 b12(b12) could recognize conformational epitopes that overlap the CD4 bs of Env. Different virus strains, even derived from the same individual, showed distinct neutralization susceptibility to b12. We examined the key amino acid residues affecting b12 neutralization susceptibility using single genome amplification and pseudovirus neutralization assay. Eleven amino acid residues were identified that affect the sensitivity of Env to b12. Through site-directed mutagenesis, an amino acid substitution at position 182 in the V2 region of Env was confirmed to play a key role in regulating the b12 neutralization susceptibility. The introduction of V182 L to a resistant strain enhanced its sensitivity to b12 more than twofold. Correspondingly, the introduction of L182 V to a sensitive strain reduced its sensitivity to b12 more than tenfold. Amino acid substitution at positions 267 and 346 could both enhance the sensitivity to b12 more than twofold. However, no additive effect was observed when the three site mutageneses were introduced into the same strain, and the sensitivity was equivalent to the single V182 L mutation. CRF07_BC is a major circulating recombinant form of HIV-1 prevalent in China. Our data may provide important information for understanding the molecular mechanism regulating the neutralization susceptibility of CRF07_BC viruses to b12 and may be helpful for a vaccine design targeting the CD4 bs epitopes.

Isolation and Characterization of Recombinant Variable Domain of Heavy Chain Anti-idiotypic Antibodies Specific to Aflatoxin B_1

Some unique subclasses of Camelidae antibodies are devoid of the light chain, and the antigen binding site is comprised exclusively of the variable domain of the heavy chain （VHH）. The recombinant VHHs have a high potential as alternative reagents for the next generation of immunoassay. In particular, they might be very useful for molecular mimicry. The present study demonstrated an alpaca immunized with the F（ab＇）z fragment of anti-aflatoxin B1 mAb and developed an important anti-idiotypic （anti-ld） responses. Antigen-specific elution method was used for panning private anti-ld VHHs from the constructed alpaca VHH library. The selected VHHs were expressed, renatured, purified, and then identified by a competitive enzyme-linked immunosorbent assay （ELISA）. Our findings indicated that the VHH would be an alternative tool for haptens mimicry studies.

The preparation of anti-hnRNP A2/B1 polyclonal antibody and its potential application in non-small cell lung cancer

Objective： In order to evaluate potential application for diagnosis and prognosis of non-small cell-lung cancer （NSCLC）, as well as to determine its role in the pathogenesis of the disease, we prepared anti-human hnRNPA2/B1 potyclonal antibody. Methods： Prokaryotic expression vector of pET28a （＋）-hnRNP A2/B1 was constructed and bansformed into E.coli BL21. The recombinant protein induced by IPTG was purified and injected to rabbits for antibody preparation. Expression of hnRN P A2/B1 was examined in 45 tissues of NSCLC and 16 inflammatory pseudotumor tissues of lung by immunohistochemistry with the antibody. The commercial hnRNP A2/B1 monoclonal antibody was used as a controI.Results： （1） Polyclonal an-tibody against hnRNP A2/B1 with high title was obtained. （2） The positive staining in NSCLC tissues was 62.22%, which was substantially higher than that in normal tissues （40%, P = 0.035） or inflammatory pseudotumor tissues （31.25%, P=0.033）. （3） Expression of hnRNP A2/B1 positively correlated with age and the history of smoking, whereas it negatively correlated with differentiation staging of tumors. （4） Follow-up study showed that the survival time of patients with positive staining was significantly shorter than that of patients without hnRNP A2/B1 expression （P=0.048）. Conclusion： It is successful to make the recombinant protein and prepare the polyclonal antibody agonist human hnRNP A2/B1. It may be a valuable marker for the diagnosis and prognosis of NSCLC. Our results provide a basis for further study in clinical application.

伏马菌素B_1免疫检测方法的研究

本研究建立了用于检测粮食、饲料中伏马菌素Ｂ１（ＦＢ１）的快速、灵敏、简便的免疫检测方法—建立在单克隆抗体基础上的直接竞争性酶联免疫吸附测定方法（ＤＣ—ＥＬＩＳＡ法）；其最低检出浓度为１０ｎｇ／ｍｌ，线性范围在１０ｎｇ～５μｇ／ｍｌ。对新疆、安徽、黑龙江、哈尔滨四省市玉米样品中的ＦＢ１含量进行了测定，结果表明１５６份样品中有３４份检出ＦＢ１，阳性率为２１．７９％，含量在０．１８～３１．３２μｇ／ｇ范围内，平均含量为１２．０４μｇ／ｇ。

抗伏马菌素B_1单克隆抗体的制备及鉴定

选择钥孔虫戚血蓝蛋白（ Ｋ Ｌ Ｈ）和牛血清白蛋白（ Ｂ Ｓ Ａ）作为半抗原伏马菌素 Ｂ１ （ Ｆ Ｂ１ ）的载体蛋白，以戊二醛一步法分别制备免疫原 Ｋ Ｌ Ｈ Ｆ Ｂ１ 和固相抗原 Ｂ Ｓ Ａ Ｆ Ｂ１ 蛋白结合物。用 Ｋ Ｌ Ｈ Ｆ Ｂ１ 免疫 Ｂａｌｂ／ｃ 小鼠后，应用细胞融合技术，筛选后获得了１株稳定分泌抗 Ｆ Ｂ１ 单克隆抗体的杂交瘤细胞株（ Ｆ Ｂ１ ４ Ｇ４ ），分泌的抗体属于 Ｉｇ Ｇ１ 亚类。腹水的抗体效价为１ｖ１×１０７ ，抗体与其它３种真菌毒素、 Ｆ Ｂ３ 和２种载体蛋白均无交叉反应，与 Ｆ Ｂ２有轻微的交叉反应。

细胞间黏附分子-1在CD4^(+)T细胞辅助B细胞产生抗体中的作用和临床意义

目的·探讨细胞间黏附分子-1(intercellular adhesion molecule-1,ICAM-1)在CD4^(+)T细胞辅助B细胞产生抗体中的作用,以及ICAM-1与系统性红斑狼疮(systemic lupus erythematosus,SLE)的相关性。方法·①选取2018年10月—2020年5月在上海交通大学医学院附属仁济医院风湿科就诊的SLE患者50例(SLE组)及仁济医院体检中心健康人60例(健康对照组,即HC组)。采用流式细胞术分析2组样本外周血CD4^(+)T细胞表面ICAM-1表达水平,酶联免疫吸附试验(enzyme-linked immunosorbent assay,ELISA)检测2组样本血清中可溶性ICAM-1(soluble ICAM-1,sICAM-1)含量。②通过密度梯度离心法分离健康人样本外周血单个核细胞,体外经α-CD3/28激活于24、48、72 h采用流式细胞术分析CD4^(+)T细胞表面ICAM-1表达水平,ELISA检测培养上清液中sICAM-1含量。③将健康人CD4^(+)T细胞-B细胞体外共培养,分别设立对照组、刺激组、阻断抗体处理组,12 d后采用ELISA检测3组培养上清液中IgG含量。结果·①SLE组外周血CD4^(+)T细胞表面ICAM-1表达水平以及血清中sICAM-1含量均较HC组升高(均P<0.05)。相关分析显示,CD4^(+)T细胞表面ICAM-1表达水平与红细胞沉降率呈正相关,血清sICAM-1含量与抗双链DNA抗体、IgG水平呈正相关(均P<0.05)。②健康人CD4^(+)T细胞表面ICAM-1表达水平和上清液中sICAM-1含量随着α-CD3/28刺激时间的延长而升高。③共培养后,刺激组上清液中IgG含量较对照组升高,而阻断抗体处理组较刺激组下降(均P<0.05)。结论·ICAM-1分子促进CD4^(+)T细胞-B细胞相互作用后IgG的产生,可作为SLE治疗的潜在靶点。

腐马素B_1单克隆抗体的制备与鉴定

本研究采用戊二醛一步法制备免疫抗原FB1 KLH和包被抗原FB1 BSA ,免疫BALB/c小鼠 ,建立间接酶联免疫吸附法 (I ELISA)并测定血清效价。结果表明 :FB1 BSA最适包被浓度为 1μg/ml,抗体最适稀释度为 1∶10 0 0 0 ,血清效价可达 1∶12 80 0 0。第 4次免疫后 ,通过淋巴细胞杂交瘤技术建立分泌FB1单克隆抗体的杂交瘤细胞株 ,融合率为 96 % ,阳性率为 98%。细胞上清抗体ELISA效价为 1∶3 2× 10 6,腹水抗体效价为 1∶8× 10 8。经鉴定 ,该株单抗的亚类为IgG1,分子量为 185 4KDa ,染色体数目介于 96～ 10 4之间 ,亲和常数为 1 16× 10 7M-1,与另三种常见的真菌毒素 (串珠镰刀菌素 ,T 2毒素 ,玉米赤霉烯酮 )和两种载体蛋白 (牛血清白蛋白 ,血蓝蛋白 )无交叉反应 。

抗黄曲霉毒素B_1蛋黄抗体的制备及其性质的研究

将黄曲霉毒Ｂ１－牛血清白蛋白（ＡＦＢ１Ｏ—ＢＳＡ）连接物免疫注射４只（Ａ、Ｂ、Ｃ、Ｄ）产蛋鸡。研究了抗ＡＦＢ１蛋黄抗体的产生进程，除鸡Ｂ外，其它３只鸡从第一次注射抗原后的第９０天开始有较明显的抗体产生，第１３５天达到高峰，从第１６５天开始下降。在抗体产生高峰期，蛋黄抗体Ａ、Ｃ、Ｄ的间接ＥＬＩＳＡ效价分别为１∶８０００、１∶６０００、１∶６０００。以蛋黄抗体Ａ为材料，研究了抗体的特异性，结果表明：该抗体有较好的特异性。但是抗体与ＡＦＢ１的结构类似物（ＡＦＢ２、ＡＦＧ２、ＡＦＧ１、ＡＦＭ１）除ＡＦＭ１外都有不同程度的交叉反应，达到５０％的竞争抑制率时，ＡＦＢ１、ＡＦＢ２、ＡＦＧ１、ＡＦＧ２的灵敏度分别为６、２５、１２５和２４９５ｎｇ／ｍｌ。

抗酪氨酸酶相关蛋白-1B细胞表位区多克隆抗体的制备及鉴定

目的 :制备多克隆抗体并初步用于TRP 1抗原表位区的研究 ,为白癜风、恶性黑素瘤的免疫治疗提供实验依据。方法 :在大肠杆菌中表达PRSETA/TRP 1融合蛋白 ,用所获得的蛋白免疫新西兰白兔得到多克隆抗体 ,并用ELISA、Western blot方法进行此抗体的鉴定。结果 :①表达了PRSETA/TRP 1融合蛋白 ;②制备了抗TRP 1B细胞表位区的多克隆抗体 ;③并用多克隆抗体检测了毕赤酵母表达的 6His TRP1蛋白 ,证实此抗体效价高、特异性强。结论 :此抗体可用于TRP

抗人B7-1人-鼠嵌合抗体体内外抑瘤作用研究

目的研究抗人B7-1人-鼠嵌合抗体ch-4E5对高表达B7-1分子的人恶性B淋巴瘤细胞株Raji的抑瘤作用。方法自行制备ch-4E5,经流式细胞术(FCM)分析ch-4E5对Raji细胞膜型B7-1分子的识别及共育后细胞表面Fas及Fas L表达的改变,继而又经MTT法检测细胞增殖的抑制效应;以人外周血PBMC为效应细胞,Raji为靶细胞,分析ch-4E5介导的抗体依赖的细胞介导的细胞毒作用(antibody dependent cell mediated cytotoxicity,ADCC);将Raji细胞经ch-4E5处理后接种Balb/c裸鼠,观察裸鼠成瘤时间并计算成瘤率。结果 ch-4E5与Raji细胞的阳性结合率为97.9%;该抗体可上调Raji表面Fas及Fas L的表达,其阳性表达率分别为15.8%及16.9%,与人Ig G1同型对照组5.1%和2.2%比较具有统计学意义(P<0.01);ch-4E5对Raji细胞增殖的抑制率为39.17%(P<0.01);介导的最大杀伤率为56.47%(P<0.01);经ch-4E5处理的Raji细胞接种Balb/c裸鼠,90 d的观察期内均未见肿瘤形成,而对照组成瘤率高达80%。结论抗人B7-1人-鼠嵌合抗体对高表达B7-1的肿瘤细胞具有抑瘤作用。

脂多糖对大鼠下丘脑室旁核GABA_BR1阳性神经元的激活作用

目的:探讨大鼠下丘脑室旁核(PVN)-氨基丁酸B受体亚单位1(GABABR1)阳性神经元对脂多糖(LPS)刺激的反应.方法:将大鼠腹腔注射LPS建立免疫应激模型,对照组注射等量的生理盐水,采用免疫荧光双标记与激光共聚焦显微镜技术,观察大鼠下丘脑室旁核内神经元Fos和GABABR1的标记情况以及它们在同一神经元内是否有共标记.结果:腹腔注射LPS可使大鼠PVN内表达Fos神经元数量显著增高,且PVN内部分神经元可同时被Fos和GABABR1双重标记,双重标记的神经元大约占Fos神经元的30%,占GAB-ABR1的24%.结论:下丘脑室旁核部分GABABR1阳性神经元参与了LPS诱导的免疫应激反应,它们可能在下丘脑-垂体-肾上腺轴的调节方面起重要作用.

人神经菌毛素1 b结构域单克隆抗体的制备及其抑制血管生成作用

目的:制备抗人神经菌毛素1(human neuropilin 1,Hu NRP1)b结构域单克隆抗体(monoclonal antibodies,m Ab),为靶向抑制肿瘤血管生成提供生物材料。方法:运用杂交瘤技术,将Hu NRP 1 b结构域重组蛋白(TF-Hu NRP1b)免疫BALB/c鼠,共免疫3次,取免疫鼠的脾脏细胞与sp2/0细胞进行融合,采用间接免疫荧光法(immunofluorescent assay,IFA)筛选稳定分泌抗Hu NRP1bm A,以Western blot、IFA、流式细胞术分析m Ab的特异性。以MTT法及小室迁移实验分析m Ab抑制血管生成的能力。结果:获得1株稳定分泌抗Hu NRP1bm Ab的细胞株4F11。Western blot结果表明,本研究所获得的m Ab 4F11只与重组Hu NRP1b发生反应,与对照蛋白不发生反应;IFA及流式细胞分析结果表明,所获得的m Ab能够识别肿瘤细胞MDA-MB-231、Hep G2以及人脐静脉内皮细胞表达的天然Hu NRP1蛋白;MTT法及小室迁移实验表明,所获得的m Ab 4F11具有抑制人脐静脉内皮细胞增殖、迁移的能力。结论:成功制备出抗Hu NRP1b的m Ab,该m Ab的获得将为进一步研究Hu NRP1的功能及靶向抑制肿瘤血管生成提供生物材料。

重组人β2糖蛋白1第一结构域二聚体作为抗磷脂抗体综合征B细胞耐受原的初步探讨

目的:探讨重组人β2糖蛋白1第一结构域二聚体(rhβ2-GP1-DⅠ2)对重组人β2糖蛋白1(rhβ2-GP1)免疫小鼠β2-GP1特异性B细胞反应的抑制作用。方法:应用固相ELISA方法,检测静脉注射rhβ2-GP1-DⅠ2后免疫小鼠产生的抗β2糖蛋白1抗体(anti-β2-GP1)滴度及anti-β2-GP1产生水平比率;应用ELISPOT方法,检测静脉注射rhβ2-GP1-DⅠ2后免疫小鼠脾脏β2-GP1特异性抗体形成细胞(AFC)数量。结果:静脉注射rhβ2-GP1-DⅠ2后,与对照组比较,rhβ2-GP1免疫小鼠βanti-β2-GP1滴度明显降低(P<0.01),anti-β2-GP1产生水平比率下降,β2-GP1特异性AFC数量明显减少(P<0.01)。结论:静脉注射rhβ2-GP1-DⅠ2能够抑制rhβ2-GP1免疫小鼠β2-GP1特异性B细胞的反应能力。

抗黄曲霉毒素B_1独特型纳米抗体的表达及复性

目的快速制备大量具有生物活性的独特型纳米抗体F7。方法构建pET22b-F7原核表达载体,转化至大肠杆菌E.coliBL21(DE3)中进行诱导表达,对诱导温度、诱导剂浓度和诱导时间进行优化。结果独特型纳米抗体F7表达量有所增加但主要以包涵体形式存在。经过包涵体的溶解、复性获得了具有生物活性的抗AFB1独特型纳米抗体,ELISA证实复性后的蛋白依然存在对鼠源AFB1抗体的结合特性。结论为后续抗体的性质研究和改造奠定了基础。

1型鸭甲肝病毒VP3蛋白的抗血清中和活性分析及B细胞表位鉴定

旨在探究1型鸭甲肝病毒(DHAV-1)VP3蛋白抗血清的中和活性并鉴定VP3的线性B细胞表位。利用pGEX-4T-1表达载体,在BL21(DE3)宿主菌中原核表达DHAV-1 VP3基因,以切胶纯化出的蛋白质为抗原免疫兔制备多克隆抗体,通过鸡胚中和试验对多抗的中和效价进行检测;采用Karplus&Schulz、Emini、Jameson-Wolf和Parker方法分别对柔韧性、表面可及性、抗原性及亲水性进行分析,得到了4条候选线性B细胞表位,以制备的兔抗VP3多克隆抗体为一抗,通过间接ELISA方法对人工合成的B细胞表位进行鉴定,并进一步用临床鸭血清样品对鉴定的B细胞表位的抗体检测能力进行评估。结果显示,VP3在BL21(DE3)中以包涵体形式表达,大小约54ku,Western blot分析表明重组蛋白质具有较好的反应原性。制备的兔抗VP3多克隆抗体的琼扩效价达到1∶16,并能中和DHAV-1,中和效价为1∶39;利用间接ELISA鉴定出GKRKPCRRPIHKPKNPPQEP(1—20aa)、FNTGRYQMSWYPIADGEQSL(131—150aa)和VNSSAPSNID(200—209aa)为VP3的B细胞表位,抗体检测能力试验结果显示表位肽可检测临床DHAV-1鸭血清。本研究表明DHAV-1VP3的抗血清具备一定的中和活性,1—20aa、131—150aa和200—209aa为VP3的B细胞表位且具有临床应用前景。

B-1细胞在牙周炎中的研究进展

牙周局部细菌感染可引发牙周组织炎症,造成牙周组织破坏,牙齿脱落。近些年,有学者发现B-1细胞占牙周炎病损部位浸润细胞的很大比例,并对B-1细胞在牙周炎中的作用进行了研究。本文就B-1细胞在牙周炎中的研究现状做一综述,以了解该领域的研究进展并为牙周炎的治疗提供新的思路。

Generation of high affinity human single-hain antibody against PreSl of hepatitis B virus from immune phage-display antibody library

BACKGROUND: A single-chain antibody ( ScFv) phage display library was created by cloning antigen-binding re- gions of VH (variable domain) and VL gene repertoires as fusion proteins with a minor coat protein of filamentous phage, from which high affinity completely humanized ScFv against PreS1 of hepatitis B virus could be screened and characterized. METHODS: A combinatorial library of phage-display hu- man ScFv genes, which were derived from peripheral blood lymphocytes immunized by peptide PreS1 in vitro, was constructed. The library contained 7 × 108 clones. RESULTS: After 3 rounds panning, a high affinity (K = 10-7-10-8 mol/L) ScFv specific to PreS1 was obtained. Sequence analysis showed that the VH belonged to the VH4 family and Vλ to Vλ4. CONCLUSIONS: The described ScFv may provide a more satisfactory therapy. This application further illustrates that the method of in vitro antigen stimulation is expeditious for the source of human immune antibody library.

Development of a QCM (Quartz Crystal Microbalance) Biosensor to the Detection of Aflatoxin B1

In this study, we have used a direct immunoassay where the simple binding between antigen and an antibody is detected. Immunoassays were performed in a drop system, monitoring the frequency decrease of the quartz-crystal microbalance device because of mass increasing during immunoreaction. The QCM sensor was coated on both sides by gold electrodes, only one side of the crystal (liquid side) was in contact with the solution;the other side (contact side) was always dry. We tested a piezoelectric immunosensor for aflatoxin B1 (AFLA-B1) mycotoxin detection through the immo- bilization of DSP-anti-AFLAB1 antibody (AFLA-B1-Ab anti AFLAB1) on gold-coated quartz crystals (AT-cut/5 MHz). The DSP (3,3’-Dithiodipropionic-acid-di-N-hydroxysuccinimide ester) was used for the covalent attachment of the proteins. The piezoelectric crystal electrodes were pretreated by DSP for 15 min, rinsed with water and dried in a gentle flow of nitrogen gas. Then the DSP-coated crystals were installed in a sample holder and exposed to the anti-AFLAB1 antibody and to the AFLA-BI. Frequency and resistance shifts (Δf and ΔR) were measured simultaneously. Δf versus AFLA-BI concentrations in the range of 0.5 - 10 ppb exhibited a perfect linear correlation with a coefficient of above 0.998.