Diphtheria Toxin/Human B-Cell Activating Factor Fusion Protein Kills Human Acute Lymphoblastic Leukemia BALL-1 Cells: An Experimental Study

Objective： This study aimed to express a fusion protein of diphtheria toxin and human B cell-activating factor （DT388sBAFF） in Escherichia coli （E. coli） and investigate its activity in human B-lineage acute lymphoblastic leukemia 1 cells （BALL-1）. Methods： A fragment of DT388sBAFF fusion gene was separated from plasmid pUC57-DT388sBAFF digested with Nde I and Xho I, and inserted into the expression vector pcold II digested with the same enzymes. Recombinants were screened by the colony polymerase chain reaction （PCR） and restriction map. The recombinant expression vector was transformed into BL21 and its expression was induced by isopropyl β-D-1-thiogalactopyranoside （IPTG）. The recombinant protein was identified by sodium dodecyl sulfate-polyacrylamide gel electrophoresis （SDS-PAGE） and Western blot, and then purified by Ni2＋-NTA affinity chromatography. The expression level of B cell-activating factor receptor （BAFF-R） on BALL-1 cells was assessed by real-time PCR. The receptor binding capacity of recombinant protein was determined by cell fluorescent assay. The specific cytotoxicity of recombinant protein on BALL-1 cells was detected by 3-（4,5-dimethylthiazolyl-2）-2,5-diphenyltetrazolium bromide （MTT） assay. Results： The expression level of recombinant protein was 50% of total bacterial proteins in E. coli, and the recombinant protein could bind to BAFF-R-positive BALL-1 cells and thereby produce a cytotoxic effect on the cells. Conclusion： The fusion protein expression vector DT388sBAFF was successfully constructed and the recombinant protein with selective cytotoxicity against BALL-1 cells was obtained, providing foundation for further study of the therapy of human B-lineage acute lymphoblastic leukemia.

Increased Expression and Activity of MMP-9 in C-reactive Protein-induced Human THP-1 Mononuclear Cells Is Related to Activation of Nuclear Factor Kappa-B

The relation between the expression and activity of MMP-9 in C-reactive protein （CRP）-induced human THP-1 mononuclear cells and the activation of nuclear factor kappa-B （NF-κB） was studied to investigate the possible role of CRP in plaque destabilization. Human THP-1 cells were incubated in the presence of CRP at 0 （control group）, 25, 50 and 100 μg/mL （CRP groups） for 24 h. In PDTC （a specific NF-κB inhibitor） group, the cells were pre-treated with PDTC at 10 μmol/L and then with 100 μg/mL CRP. The conditioned media （CM） and human THP-1 cells in different groups were harvested. MMP-9 expression in CM and human THP-1 cells was measured by ELISA and Western blotting. MMP-9 activity was assessed by fluorogenic substrates. The expression of NF-κB inhibitor α （IκB-α） and NF-κB p65 was detected by Western blotting and ELISA respectively. The results showed that CRP increased the expression and activity of MMP-9 in a dose-dependent manner in the human THP-1 cells. Western blotting revealed that IiB-α expression was decreased in the cells with the concentrations of CRP and ELISA demonstrated that NF-κB p65 expression in the CRP-induced cells was increased. After pre-treatment of the cells with PDTC at 10 μmol/L, the decrease in IκB-α expression and the increase in NF-κB p65 expression in the CRP-induced cells were inhibited, and the expression and activity of MMP-9 were lowered too. It is concluded that increased expression and activity of MMP-9 in CRP-induced human THP-1 cells may be associated with activation of NF-κB. Down-regulation of the expression and activity of MMP-9 may be a new treatment alternative for plaque stabilization by inhibiting the NF-κB activation.

ESTABLISHMENT OF A HUMAN B CELL LINE THAT RESPONDS SPECIFICALLY TO B CELL GROWTH FACTOR

A human B cell line （3D5） that responds specifically to B cell growth factor （BCGF） hasbeen developed by a sequence of Staphylococcus aureus Cowen I activation,EB virus im-mortalization,and cloning.Proliferative response to PHA-stimulated T cell supernatant（PHA-T-Sup） and nonresponsiveness to rIL-2 stimulation were factors used to screen positivecells.Phenotype analysis with a flow cytometer indicated that:1) 3D5 is a B cell line:100% of the cells were positive for B1 marker and 59% were positive for sIg,while T3and Mo 1 were negative:2) 3D5 is an activated B cell line:both Tac and 4F2 markersof activated （but not of resting） B cells were 100% positive:3) 3D5 expresses high molecularweight BCGF （HMW-BCGF） receptor-associated epitope BA5.3D5 cells proliferated inresponse to cpBCGF stimulation in a dose-dependent manner.HMW-BCGF also induced3D5 cells to proliferate.Interestingly.no proliferation could be detected in the presenceof rIL-2,rIL-4,or rIFN-r.The data show that 3D5 cells are specifically BCGF-responsiveB cells.Using 3D5 cells as target,BCGF activity was detected in crude BCGF preparationsedimented by 85% （NH4）2SO4 and chromatographed in a DEAE-Sephadex A-25 column fromPHA-T-Sup.T24 cell supernatant with B cell differentiation factor （BCDF） activity couldnot induce 3D5 cells to differentiate into immunoglobulin-secreting cells.

Influence of baicalin on the expression of receptor activator of nuclear factor-κB ligand and osteoprotegerin in human periodontal ligament cells

Objective To study the effect of baicalin on the expression of receptor activator of nuclear factor-κB ligand(RANKL)and osteoprotegerin(OPG)in cultured human periodontal ligament(HPDL)cells.Methods Small interfering RNA(siRNA)eukaryotic expression vector targeted transforming growth factor βⅡ receptor(TGF-β RⅡ)was constructed and transfected into T cells.HPDL cells with T cells transfected with siRNA or not were placed in the culture medium that had been added with lipopolysaccharide(LPS)and baicalin.The obtained solution was divided into six groups according to the components(group Ⅰ:HPDL cells+LPS+T cells transfected with siRNA1+baicalin;group Ⅱ:HPDL cells+LPS+T cells transfected with siRNA1;group Ⅲ:HPDL cells+LPS+T cells+baicalin;group Ⅳ:HPDL cells+LPS+T cells;group Ⅴ:HPDL cells+baicalin;group Ⅵ:HPDL cells)and was cultured for 48 hours.RT-PCR was used to observe the effect of baicalin on the expression of OPG-RANKL in HPDL cells.Results The ratio of RANKL/OPG in group Ⅰ was lower than that in group Ⅱ(P<0.01)and higher than that in group Ⅲ(P<0.01);The ratio of RANKL/OPG in group Ⅲ was lower than that in group Ⅳ(P<0.01);the ratio of RANKL/OPG in group Ⅳ was higher than that in group Ⅵ(P<0.01);the ratio of RANKL/OPG in group Ⅴ was lower than that in group Ⅵ(P<0.05).Conclusion ① Baicalin could decrease the ratio of RANKL/OPG in HPDL cells.② The TGF-β signaling transduction plays an important role in the effect of baicalin on the RANKL/OPG ratio in HPDL cells.③ Baicalin acts not only through TGF-β to regulate RANKL/OPG in HPDL cells,but also through other pathways.

CONDITIONED MEDIUM OF HUMAN NASOPHARYNGEAL CARCINOMA EPITHELIOID CELL LINE CNE_(1) CONTAINED THE ACTIVITIES OF TRANSFORMED GROWTH-INHIBITING FACTORS

The hormone defined serum free conditioned medium (SFCM) of human nasopharyngeal carcinoma epithelioid cell line (CNE1) was assayed by both the 3H-thymidine incorporation test and the soft agar test. It was found that the SFCM stimulated the growth of long-term serum-free cultured CNE4 cells in ac-cordence with the fact that the growth rate of long-term serum-free cultured CNE1 cells was directly proportional to the plating density. Alternatively 5% SFCM inhibited the growth of short-term serum-free cultured CNE4 cells by 51% in which the indicator cell remained the responsiveness state of growing in the serum-supplemented medium to the effector of interest. Furthermore, SFCM resulted in the inhibition of anchorage-independent growth of CNE4 cells and A431 cells. Also in soft agar test. SFCM reduced the colony formation of NRK(?),9F cells in the presence of EGF or EGF plus TGF-β. These finding suggested that CNE4 secreted autocrine growth stimulating factor(s) and growth inhibiting factor(s) in the serum-free medium, the latter strongly reverse malignant phenotypes of CNE4 and A431 cells in serum-supplemented surrounding.

BAFF调节免疫性血小板减少症模型小鼠的Th17/Treg平衡的研究

目的:探讨B细胞激活因子(BAFF)对免疫性血小板减少症模型小鼠体内辅助性T细胞17(Th17)/调节性T细胞(Treg)平衡的调节作用和潜在机制。方法:制备豚鼠抗小鼠血小板抗血清(GP-APS),并将150只无特定病原级别的成年雄性BALB/c小鼠(7~8周龄)随机分为5组,每组30只。分别为对照组(空白对照)和ITP组(GP-APS诱导),ITP+rhBAFF组(ITP组联合静脉注射50μg/kg/50μL重组人BAFF蛋白),并在ITP+rhBAFF组处理的基础上分别联合Notch1的抑制剂(DAPT)或PI3K/Akt的抑制剂Polygalacin D(PGD),设立ITP+rhBAFF+DAPT组和ITP+rhBAFF+PGD组,除对照组和ITP组外,均为静脉注射给药,DAPT注射剂量100μg/kg;PGD注射剂量25μg/kg,静脉注射总体积均为50μL,每日1次。1周后取小鼠1mL外周血并分离血清和单个核细胞。用免疫荧光化学检测单个核细胞中BAFF和Notch1的定位。对外周血中的血小板进行计数。酶联免疫吸附法(ELSIA)检测小鼠外周血血清BAFF的水平。Western blot检测小鼠外周血单个核细胞中PI3K、AKT、Notch1、p-Akt(Thr308)、p-Akt(Ser473)的蛋白表达。流式细胞术检测单个核细胞中Th17/Treg的比例变化。结果:ITP小鼠外周血单个核细胞的BAFF与Notch1共定位在细胞膜。与对照组比较,ITP组BAFF、Notch1、p-Akt(Thr308)、p-Akt(Ser473)的表达增加,血小板数目和Treg比例减少,Th17比例增加(P<0.05)。与ITP组比较,ITP+rhBAFF组BAFF、Notch1、p-Akt(Thr308)、p-Akt(Ser473)的表达增加,血小板数目和Treg比例减少,Th17比例增加(P<0.05)。与ITP+rhBAFF组比较,ITP+rhBAFF+DAPT组BAFF、Notch1、p-Akt(Thr308)、p-Akt(Ser473)的表达降低,血小板数目和Treg比例增加,Th17比例降低(P<0.05)。与ITP+rhBAFF组比较,ITP+rhBAFF+PGD组BAFF、Notch1、p-Akt(Thr308)、p-Akt(Ser473)的表达降低,血小板数目和Treg比例增加,Th17比例降低(P<0.05)。结论:BAFF通过激活Notch1/PI3K/Akt信号通路促进免疫性血小板减少症模型小鼠体内Th17比例增加及Treg比例减少。

B细胞活化因子与小儿自身免疫性脑炎严重程度的相关性分析

目的分析B细胞活化因子(BAFF)与小儿自身免疫性脑炎严重程度的相关性,为临床诊治小儿自身免疫性脑炎提供思路。方法该研究采用病例-对照的研究方法,将该院2020年1月至2022年6月收治的45例自身免疫性脑炎患儿作为病例组,另将该院同期收治的45例病毒性脑炎患儿作为对照组;查阅两组患儿电子病历档案,收集性别、年龄、临床特征、脑脊液BAFF、血清BAFF等临床资料;应用改良Rankin量表(mRS)评估自身免疫性脑炎患儿的病情严重程度,比较轻度组、中重度组患儿实验室资料及影像学资料,分析BAFF与小儿自身免疫性脑炎严重程度的关系。结果病例组临床特征为精神行为异常、认知障碍、癫痫发作、语言障碍、意识障碍占比高于对照组,临床特征为发热、恶心占比低于对照组,差异有统计学意义(P<0.05);病例组脑脊液BAFF及血清BAFF水平低于对照组,差异有统计学意义(P<0.05);病例组与对照组其他资料对比,差异无统计学意义(P>0.05);45例自身免疫性脑炎患儿经评估,病情程度为轻度28例,中重度17例;轻度组白细胞计数、中性粒细胞计数、mRS评分低于中重度组,白蛋白、脑脊液BAFF及血清BAFF水平高于中重度组,差异有统计学意义(P<0.05);其他不同病情程度患儿实验室资料及影像学资料对比,差异无统计学意义(P>0.05);经Point-biserial相关性分析显示,脑脊液BAFF及血清BAFF与小儿自身免疫性脑炎严重程度均呈负相关(r=-0.524、-0.562,P<0.05);经Pearson相关性分析显示,自身免疫性脑炎患儿脑脊液BAFF与血清BAFF呈正相关(r=0.437,P<0.05);绘制受试者工作特征曲线,结果显示,脑脊液BAFF、血清BAFF预测小儿自身免疫性脑炎严重程度的曲线下面积均>0.7,均具有良好的预测价值。结论BAFF与小儿自身免疫性脑炎严重程度密切相关,且对预测小儿自身免疫性脑炎严重程度具有良好的价值。

Competition between TRAF2 and TRAF6 Regulates NF-κB Activation in Human B Lymphocytes

Objective To investigate the role of TNF receptor-associated factor 2 (TRAF-2) and TRAF6 in CD40-induced nuclear factor-κB (NF-κB) signaling pathway and whether CD40 signaling requires TRAF2. Methods Human B cell lines were transfected with plasmids expressing wild type TRAF2 or dominant negative TRAF2,TRAF2-shRNA,or TRAF6-shRNA. The activation of NF-κB was detected by Western blot,kinase assay,transfactor enzyme-linked immunosorbent assay (ELISA),and fluorescence resonance energy transfer (FRET). Analysis of the role of TRAF-2 and TRAF-6 in CD40-mediated NF-κB activity was examined following stimulation with recombinant CD154. Results TRAF2 induced activity of IκB-kinases (IKKα,IKKi/ε),phosphorylation of IκBα,as well as nuclear translocation and phosphorylation of p65/RelA. In contrast,TRAF6 strongly induced NF-κB activation and nuclear translocation of p65 as well as p50 and c-Rel. Engagement of CD154-induced nuclear translocation of p65 was inhibited by a TRAF6-shRNA,but conversely was enhanced by a TRAF2-shRNA. Examination of direct interactions between CD40 and TRAFs by FRET documented that both TRAF2 and TRAF6 directly interacted with CD40. However,the two TRAFs competed for CD40 binding. Conclusions These results indicate that TRAF2 can signal in human B cells,but it is not essential for CD40-mediated NF-κB activation. Moreover,TRAF2 can compete with TRAF6 for CD40 binding,and thereby limit the capacity of CD40 engagement to induce NF-κB activation.

Effects of transforming growth factor β2 and connective tissue growth factor on induction of epithelial mesenchymal transition and extracellular matrix synthesis in human lens epithelial cells

AIM:To Investigate the effects of transforming growth factorβ2(TGF-β2)and connective tissue growth factor(CTGF)on transdifferentiation of human lens epithelial cells(HLECs)cultured in vitro and synthesis of extracellular matrix(ECM).METHODS:HLECs were treated with TGF-β2(0,0.5,1.0,5,10μg/L)and CTGF(0,15,30,60,100μg/L)for different times(0,24,48,72h)in vitro and the expression ofα-smooth muscle actin(α-SMA),the main component of the extracellular matrix typeⅠcollagen(Col-1)and fibronectin(Fn)were measured by using real-time polymerase chain reaction(PCR)and western-blot.RESULTS:TGF-β2 and CTGF significantly increased expression ofα-SMA mRNA and protein(P【0.05,P【0.001),Fn mRNA and protein(P【0.001),Col-1 mRNA and protein(P【0.001).TGF-β2 could induce HLECs expression of CTGF mRNA and protein in dosedependent manner(P【0.05,P【0.001).TGF-β2 and CTGF could induce HLECs to expressα-SMA,Fn and Col-1 in time-dependent manner.Each time of TGF-β2and CTGF induced HELCs expression ofα-SMA,Fn,Col-1 mRNA and protein was significant increase compared with control(P【0.05,P【0.001).CONCLUSION:TGF-β2 and CTGF could induce HLECs epithelial mesenchymal transition and ECM synthesis.

B细胞激活因子及其靶向药物与炎症性肠病的研究进展

B细胞激活因子(B-cell activating factor,BAFF)作为B细胞的关键调节因子,参与多种自身免疫性疾病。炎症性肠病(inflammatory bowel disease,IBD)是一组病因尚不明确的慢性、反复发作的肠道炎症性疾病,近年来全球发病率呈上升趋势。多种因素引起的异常免疫反应与IBD发病密切相关,B细胞异常活化及自身抗体产生增加在溃疡性结肠炎的发病中已得到证实,而BAFF是否参与IBD发病机制尚不明确。该文就目前关于BAFF在IBD发病机制中的潜在作用以及在IBD中针对BAFF的靶向治疗研究进行综述,旨在为IBD靶向治疗提供思路。

生腺布液汤对干燥综合征NOD小鼠B细胞活化因子及B细胞活化因子受体表达的影响

目的:观察生腺布液汤对干燥综合征(SS)NOD模型小鼠颌下腺及血清中B细胞活化因子(BAFF)及B细胞活化因子受体(BAFFR)的影响,探索生腺布液汤治疗SS的作用机制。方法:将24只8周龄雌性NOD小鼠随机分为模型组、硫酸羟氯喹组及生腺布液汤组,每组8只,另取8只同周龄雌性BALB/c小鼠设为正常对照组。给药组分别予生腺布液汤1.75 g/ml灌胃及硫酸羟氯喹溶液0.0026 g/ml灌胃,模型组及正常组予等量蒸馏水,连续8周。实验期间记录小鼠的一般情况及每日饮水量;HE染色观察各组小鼠颌下腺组织病理变化;免疫组化法检测颌下腺组织BAFF、BAFFR表达;ELISA法检测血清BAFF含量。结果:与模型组相比,生腺布液汤组和硫酸羟氯喹组小鼠饮水量下降(均P<0.05),血清BAFF及颌下腺组织BAFF、BAFFR表达降低(均P<0.05),颌下腺组织中淋巴细胞浸润减少,未见明显浸润灶等组织结构破坏。结论:生腺布液汤能够改善干燥综合征NOD小鼠口干症状,减轻颌下腺淋巴细胞浸润程度,其作用机制可能与降低颌下腺及血清BAFF、BAFFR表达相关。

孕早期监测BAFF、AMH、IL-2预测复发性流产患者流产再发生的临床价值

目的探究孕早期监测B淋巴细胞活化因子(BAFF)、抗米勒管激素(AMH)、白介素-2(IL-2)对复发性流产患者流产再发生的临床预测价值。方法选取2019年9月至2023年6月上海健康医学院附属崇明医院收治的100例复发性流产患者作为研究对象并纳入观察组,根据患者早期妊娠情况分为非流产组(n=65)和流产组(n=35);选取同期同院100例产检健康的孕妇作为对照组。比较各组血清BAFF、AMH、IL-2水平,分析BAFF、AMH、IL-2水平预测流产再发生的临床价值。采用Logistic回归分析影响复发性流产患者流产再发生的因素。结果观察组BAFF、IL-2水平比对照组高,AMH水平比对照组低(P<0.05)。流产组BAFF、IL-2水平比非流产组高,AMH水平比非流产组低(P<0.05)。流产组孕次、流产≥3次比例高于非流产组(P<0.05)。绘制受试者工作特征(ROC)曲线发现,BAFF、AMH、IL-2水平预测患者发生再流产的曲线下面积(AUC)分别是0.809、0.821、0.803,三者联合检测的AUC为0.919,均优于各自单独检测(Z=1.920、1.974、2.298,P<0.05)。多因素Logistic回归发现,BAFF、IL-2是影响患者发生再流产的危险因素,AMH为保护因素(P<0.05)。结论复发性流产患者BAFF、IL-2水平升高,AMH水平降低,且三者联合检测有助于早期预测流产再发生,具有一定的诊断价值。

B细胞活化因子/增殖诱导配体对特发性炎性肌病B细胞影响的研究进展

特发性炎性肌病(idiopathic inflammatory myopathies,IIM)是免疫介导肌肉炎症为主要特征的系统性自身免疫性疾病。淋巴细胞是IIM发病机制中的关键免疫调节细胞,可引起自身免疫和炎症反应。B细胞活化因子(B cell activating factor,BAFF)/增殖诱导配体(a proliferation-inducing ligand,APRIL)是肿瘤坏死因子超家族成员,BAFF/APRIL通过与相应受体结合,影响B细胞的增殖、成熟和分化,浆细胞的存活,免疫球蛋白类别的转换,从而调控免疫反应。研究发现,BAFF/APRIL参与多种自身免疫性疾病的发病机制,与IIM发生和发展密切相关,文章对BAFF/APRIL在IIM的研究进展进行综述。

芪地桃蛭二蝉方联合他克莫司治疗膜性肾病的效果及对血清PLA2R、BAFF、IL-6水平的影响

目的 探究芪地桃蛭二蝉方联合他克莫司治疗膜性肾病的效果及对抗磷脂酶A2受体(PLA2R)、B淋巴细胞活化因子(BAFF)及白细胞介素-6(IL-6)水平的影响。方法 选取2017年11月至2020年4月收治的84例膜性肾病患者为研究对象,将其随机分为对照组与联合组,各42例。对照组给予基础治疗加他克莫司治疗,联合组在对照组基础上加芪地桃蛭二蝉方治疗。比较两组的治疗效果。结果 联合组的治疗总有效率高于对照组,差异具有统计学意义(P<0.05)。治疗前,两组的24 h尿蛋白定量(24 h UPQ)、人血清白蛋白(HSA)、血清肌酐浓度(Scr)水平比较,差异无统计学意义(P>0.05);治疗后,两组的24 h UPQ、Scr水平均明显降低,HSA水平均明显升高,且联合组优于对照组,差异具有统计学意义(P<0.05)。治疗前,两组的PLA2R、BAFF及IL-6水平比较,差异无统计学意义(P>0.05);治疗后,两组的PLA2R、BAFF及IL-6水平均明显降低,且联合组低于对照组,差异具有统计学意义(P<0.05)。联合组的不良反应总发生率低于对照组,差异具有统计学意义(P<0.05)。结论 芪地桃蛭二蝉方联合他克莫司治疗膜性肾病效果显著,能够明显降低PLA2R、BAFF及IL-6水平,安全可靠,值得推广。

Double potentialities of tumoricide and hematopoiesis of human bone marrow cells activated by IL-2 and IL-3

The biomodulative and hematopoietic potentialities of IL-2 and IL-3 activatedbone marrow(ABM)cells from patients with lung adenocarcinoma were studied in vitro.Human bone marrow(BM)cells could be activated by IL-2 in culture for 7d.TheseIL-2 ABM cells had higher cytolytic activities against cells of H 7402 cell line and freshautologous adenocarcinoma cells and maintained the cytotoxicities longer than IL-2 acti-vated peripheral blood lymphocytes(APBLs),a point of possible importance in adoptiveimmunotherapy for cancer patients.The IL-2 ABM cells also had similar number ofBFU-E and CFU-GM to that had fresh BM cells if 1L-3 was added 48h alter IL-2 inculture.The IL-2 and IL-3 ABM cells might be used to eliminate tumor cells and tosupply reconstitutive elements of BM for autologous bone marrow transplantation.

Antiretroviral naive and treated patients: Discrepancies of B cell subsets during the natural course of human immunodeficiency virus type 1 infection

AIM To evaluate alterations of memory B cell subpopulations during a 48-wk period in human immunodeficiency virus type 1(HIV-1) patients. METHODS Forty-one antiretroviral na?ve and 41 treated HIV-1 patients matched for age and duration of HIV infection were recruited. All clinical, epidemiological and laboratory data were recorded or measured. The different B cell subsets were characterized according to their surface markers: Total B cells(CD19^+), memory B cells(CD19^+CD27^+, BMCs), resting BMCs(CD19^+CD27^+CD21^(high), RM), exhausted BMCs(CD19^+CD21^(low)CD27-, EM), IgM memory B(CD19^+CD27^+IgM^(high)), isotype-switched BMCs(CD19^+CD27^+IgM-, ITS) and activated BMCs(CD19^+CD21^(low+)CD27^+, AM) at baseline on week 4 and week 48.RESULTS Mean counts of BMCs were higher in treated patients. There was a marginal upward trend of IgM memory B cell proportions which differed significantly in the treated group(overall trend, P = 0.004). ITS BMC increased over time significantly in all patients. Naive patients had of ^(low)er levels of EM B cells compared to treated, with a downward trend, irrespectively of ^(high)ly active antiretroviral therapy(HAART) intake. Severe impairment of EM B cells was recorded to both treated(P = 0.024) and naive(P = 0.023) and patients. Higher proportions of RM cells were noted in HAART group, which differed significantly on week 4^(th)(P = 0.017) and 48th(P = 0.03). Higher levels of AM were preserved in HAART naive group during the whole study period(week 4: P = 0.018 and 48: P = 0.035). HIV-RNA viremia strongly correlated with AM B cells(r = 0.54, P = 0.01) and moderately with RM cells(r =-0.45, P = 0.026) at baseline.CONCLUSION HIV disrupts memory B cell subpopulations leading to impaired immunologic memory over time. BMC, RM, EM and ITS BMC were higher in patients under HAART. Activated BMCs(AM) were higher in patients without HAART. Viremia correlated with AM and RM. Significant depletion was recorded in EM B cells irrespectively of HAART intake. Perturbations in BMC-populations are not fully restored by antiretrovirals.

淋巴样增强结合因子1在B细胞慢性淋巴增殖性疾病中的表达

目的研究淋巴样增强结合因子1(lymphoid enhancer-binding factor 1,LEF1)在B细胞慢性淋巴增殖性疾病(B cell chronic lymphoproliferative disorders,B-CLPD)中的表达情况,探讨在B-CLPD亚型诊断中的价值。方法回顾性分析58例B-CLPD患者骨髓或淋巴结标本和20例对照组标本,采用免疫组化的方法,检测LEF1的表达情况。结果慢性淋巴细胞白血病(chronic lymphocytic leukemia,CLL)20例,LEF1阳性16例,阳性率为80%;套细胞淋巴瘤阳性为1/12;滤泡性淋巴瘤为1/5;边缘区淋巴瘤为0/11;淋巴浆细胞淋巴瘤为0/8;毛细胞白血病0/2;20例非恶性血液病患者未见LEF1表达;LEF1表达在CLL组差异有统计学意义(P=0.000);LEF1的表达和CD200、CLL积分等CLL的相关指标具有相关性(P<0.05)。4例LEF1阴性的CLL患者中,2例+12染色体异常,检出率高于LEF1阳性组(P>0.05)。结论LEF1在慢性淋巴细胞白血病患者的诊断和鉴别诊断中,有较好的灵敏性和特异性,是B-CLPD鉴别诊断的良好指标。

尿石素B对骨髓来源巨噬细胞向破骨细胞分化的调控机制

背景:尿石素B在机体免疫应答中起重要调节作用,具备抗炎、抗氧化和抗癌的特性,并能抑制Raw 264.7细胞向破骨细胞分化,但其对于骨髓来源的巨噬细胞向破骨细胞分化的具体作用及机制尚未阐明。系统性研究破骨细胞过度活化的调控机制,有助于探索新的治疗靶点,筛选研发更安全、有效的治疗药物,为阻断破骨细胞过度活化提供新思路。目的:利用骨髓来源的巨噬细胞建立体外破骨细胞分化模型,探究尿石素B对核因子κB受体活化因子配体介导破骨细胞分化的影响,并系统性分析其作用机制。方法:(1)采用CCK-8法筛选尿石素B干预骨髓来源巨噬细胞的安全工作浓度;(2)用不同浓度(0,12.5,25,50μmol/L)尿石素B干预骨髓来源的巨噬细胞向破骨细胞分化,进行抗酒石酸酸性磷酸酶染色观察破骨细胞的数目及面积大小;(3)不同浓度(0,12.5,25,50μmol/L)尿石素B干预骨髓来源巨噬细胞的破骨分化,通过实时荧光定量PCR检测破骨特异性基因的相对表达水平;(4)蛋白印迹实验观察尿石素B对骨髓来源巨噬细胞P65、ERK信号通路的影响;(5)蛋白印迹实验检测尿石素B对骨髓来源巨噬细胞的破骨分化关键转录因子活化T细胞核因子1和c-Fos的影响。结果与结论:(1)50μmol/L及以下浓度的尿石素B对骨髓来源巨噬细胞的增殖无影响,能显著抑制骨髓来源巨噬细胞的破骨分化;(2)尿石素B主要在破骨形成前中期抑制骨髓来源巨噬细胞的破骨分化;(3)尿石素B可下调骨髓来源巨噬细胞中破骨特异性基因的相对表达水平;(4)50μmol/L的尿石素B抑制骨髓来源巨噬细胞的P65和ERK磷酸化水平,进而抑制破骨细胞形成;(5)50μmol/L的尿石素B抑制骨髓来源的巨噬细胞中破骨分化关键转录因子活化T细胞核因子1和c-Fos的表达;(6)提示尿石素B通过P65/ERK信号轴下调破骨关键转录因子活化T细胞核因子1、c-Fos的表达,抑制下游破骨特异性基因的表达,从而抑制骨髓来源的巨噬细胞向破骨细胞分化。

血清MBL、BAFF与磷脂酶A2受体相关特发性膜性肾病患者肾功能及疗效的关系

目的探讨血清甘露聚糖结合凝集素(MBL)、肿瘤坏死因子家族B细胞活化因子(BAFF)与磷脂酶A2受体(PLA2R)相关特发性膜性肾病(IMN)患者肾功能和疗效的关系。方法选取PLA2R相关IMN患者103例作为观察组,并根据疗效将PLA2R相关IMN患者分为未缓解组(n=44)、缓解组(n=59);同期另选健康体检志愿者67例作为对照组。收集相关资料;用酶联免疫吸法检测血清MBL、BAFF、24 h尿蛋白,PA速率微板法试剂盒检测血肌酐,计算估计肾小球滤过率(eGFR)。Spearman相关法分析PLA2R相关IMN患者血清MBL、BAFF水平与肾功能指标的相关性;多因素Logistic回归分析影响PLA2R相关IMN患者疗效的因素,受试者工作特征(ROC)曲线分析血清MBL、BAFF对PLA2R相关IMN患者治疗未缓解的预测价值。结果观察组血清MBL、BAFF水平及24 h尿蛋白高于对照组,eGFR低于对照组(P均<0.05)。PLA2R相关IMN患者血清MBL、BAFF水平与eGFR呈负相关(r分别为-0.777、-0.760,P均<0.05),与24 h尿蛋白呈正相关(r分别为0.883、0.828,P均<0.05)。未缓解组白蛋白、eGFR低于缓解组,24 h尿蛋白、MBL、BAFF高于缓解组(P均<0.05),两组性别、年龄、血肌酐、血尿酸、血尿素氮、总胆固醇、甘油三酯、IgG、补体3和PLA2R抗体滴度比较差异无统计学意义(P均>0.05)。白蛋白和eGFR升高为PLA2R相关IMN患者疗效的独立保护因素(P均<0.05),24 h尿蛋白、MBL和BAFF升高为独立危险因素(P均<0.05)。ROC曲线分析结果显示,血清MBL、BAFF联合预测PLA2R相关IMN患者治疗未缓解的曲线下面积(0.880)大于二者单独预测(0.791、0.787),比较差异有统计学意义(Z分别为2.694、2.613,P均<0.05)。结论血清MBL、BAFF水平升高与PLA2R相关IMN患者肾功能降低及疗效差有关,二者联合检测预测PLA2R相关IMN患者治疗未缓解的价值较高。

血清B细胞活化因子水平与ST段抬高型心肌梗死患者心血管事件的相关性研究

目的 评估血清B细胞活化因子(BAFF)水平对ST段抬高型心肌梗死(STEMI)患者心血管事件的预测价值。方法 选取2020年1月—2022年6月在南通大学附属南通第三医院因STEMI入院并接受冠状动脉造影的166例患者为研究对象,收集患者的一般资料、病史、超声心动图和实验室数据。对患者随访12个月,记录主要不良心血管事件(MACE)发生情况。采用Cox比例风险模型评估血清BAFF水平对MACE的预测价值;绘制血清BAFF水平预测MACE的受试者工作特征(ROC)曲线,并计算曲线下面积(AUC)。通过ROC曲线确定血清BAFF水平的最佳截断值,依照最佳截断值进行分组,采用Log-rank检验绘制Kaplan-Meier曲线以分析MACE发生情况。结果 166例患者中,26例患者在随访12个月内出现MACE, MACE发生率为15.7%。MACE组患者年龄、甘油三酯、低密度脂蛋白、心肌肌钙蛋白I、肌酸激酶同工酶、血清BAFF水平高于非MACE组患者,差异有统计学意义(P<0.05)。Cox比例风险模型结果显示,年龄与MACE发生率呈显著正相关(HR=1.267, 95%CI:1.126~1.426,P<0.001),血清BAFF水平与MACE发生率呈显著正相关(HR=1.020, 95%CI:1.003~1.038,P=0.024)。血清BAFF水平预测MACE发生率的敏感度为76.2%,特异度为82.9%。ROC曲线分析显示血清BAFF水平的最佳截断值为1.07 ng/mL,据此将患者分为血清BAFF水平>1.07 ng/mL组和血清BAFF水平≤1.07 ng/mL组,结果显示血清BAFF水平≤1.07 ng/mL组患者累积生存率高于血清BAFF水平>1.07 ng/mL组患者,差异有统计学意义(P<0.001)。结论 血清BAFF水平升高与STEMI患者MACE发生率增高呈显著正相关,血清BAFF水平能够作为STEMI患者心血管事件的预测因子。