老年急性进展性脑梗死患者血清磷脂酶A2、S100钙结合蛋白B水平与颈动脉斑块的联系

目的探讨老年急性进展性脑梗死患者血清磷脂酶A2(PLA2)、S100钙结合蛋白B(S100B)和颈动脉斑块的关系。方法将2021年1月至2022年6月收治的120例老年急性进展性脑梗死患者纳入观察组,同期将115例非进展性脑梗死患者为非进展组,100例健康人员为健康组。将观察组分为无斑块组34例、斑块稳定组45例和斑块不稳定组41例。分析血清PLA2、S100B水平与颈动脉斑块的关系。ROC分析二者对颈动脉斑块的预测价值。随访1年,以复发和死亡为终点事件分析生存率。结果斑块稳定组、斑块不稳定组血清PLA2、S100B高于无斑块组,差异有统计学意义(P<0.05)。血清PLA2、S100B与颈动脉斑块呈正相关。ROC显示二者联合预测的价值更高(P<0.05)。结论血清PLA2、S100B在老年急性进展性脑梗死患者水平升高,与颈动脉斑块关系密切。

温阳益髓方联合富血小板血浆治疗早中期膝骨关节炎的疗效及对血清S100B、CTX-Ⅱ水平的影响

目的 分析温阳益髓方联合富血小板血浆(PRP)治疗早中期膝骨关节炎(KOA)的疗效及对血清S100B、Ⅱ型胶原C端肽(CTX-Ⅱ)水平的影响。方法 选取2021年4月至2023年1月该院收治的150例早中期KOA患者作为研究对象,根据随机数字表法将其分为观察组和对照组,各75例。对照组给予PRP治疗,观察组在对照组基础上联合温阳益髓方治疗。对比两组临床疗效、不良反应总发生率、复发率,治疗前、治疗1个月后Lysholm膝关节功能量表(LKS)评分,血清S100B、CTX-Ⅱ水平,以及治疗前、治疗1周、1个月后视觉模拟评分法(VAS)评分。结果 观察组总有效率高于对照组,复发率低于对照组,差异均有统计学意义(P<0.05)。治疗1个月后两组LKS评分高于治疗前,且观察组LKS评分高于对照组,差异均有统计学意义(P<0.05)。重复测量方差分析显示,两组治疗期间VAS评分变化有交互效应(F=20.132,P=0.030),故进一步做单独交应分析,对照组和观察组治疗1周、1个月后的VAS评分均低于治疗前,且治疗1个月后的VAS评分低于治疗1周后,差异均有统计学意义(P<0.05)。多变量方差分析结果显示,治疗1周、1个月后观察组VAS评分低于对照组,差异均有统计学意义(P<0.05)。治疗1个月后两组血清S100B、CTX-Ⅱ水平低于治疗前,且观察组低于对照组,差异均有统计学意义(P<0.05)。两组不良反应总发生率比较,差异无统计学意义(P>0.05)。结论 温阳益髓方联合PRP治疗早中期KOA患者的临床效果显著,可有效缓解疼痛症状,改善血清S100B、CTX-Ⅱ水平,促进膝关节功能康复,降低疾病复发率,值得临床推广。

Soluble Structure of CLIC and S100 Proteins Investigated by Atomic Force Microscopy

The ability to visualise proteins in their native environment and discern information regarding stoichiometry is of critical importance when studying protein interactions and function. We have used liquid cell atomic force microscopy (AFM) to visualise proteins in their native state in buffer and have determined their molecular volumes. The human proteins S100A8, S100A9, S100A12 and CLIC1 were used in this investigation. The effect of oxidation on the protein structure of CLIC1 was also investigated and we found that CLIC1 multimerisation could be discerned by AFM, which supports similar findings by other methods. We have found good correlation between the molecular volumes measured by AFM and the calculated volumes of the individual proteins. This method allows for the study of single soluble proteins under physiological conditions and could potentially be extended to study the structure of these proteins when located within a membrane environment.

人参黄芩配伍通过调控S100B信号通路对下肢动脉硬化闭塞症大鼠内皮细胞功能、氧化应激的影响

目的 探究人参黄芩配伍通过调控钙结合蛋白(S100B)信号通路对下肢动脉硬化闭塞症大鼠内皮细胞功能、氧化应激的影响。方法 选取40只SPF级SD雄性大鼠,随机分为正常(N)组、模型(M)组、曲美他嗪(T)组、人参黄芩配伍(G)组各10只,对M、E、G组采用高脂饮食加隐动脉内膜损伤法建立下肢动脉硬化闭塞症模型,N组不建立该模型,建模成功后,对T组灌胃30 mg/kg曲美他嗪,对G组灌胃2 g/kg人生黄芩,N组、M组同期灌胃同体积生理盐水,塔洛夫(Tarlov)评分评价大鼠下肢运动功能,苏木素-伊红(HE)染色法检测血管组织病理形态,酶联免疫吸附试验(ELISA)检测内皮细胞功能相关指标,黄嘌呤氧化酶法和硫代巴比妥酸法检测氧化应激相关指标,Western印迹检测S100B信号通路相关蛋白表达。结果 与N组比较,M组Tarlov评分明显降低(P<0.05);与M组比较,T、G两组Tarlov评分均明显升高(P<0.05);且与T组相比,G组升高显著(P<0.05);N组血管结构清晰完整,血管内皮细胞无增生及脱落,未见动脉硬化斑块及炎性细胞浸润,M组动脉壁各层分界不清,血管壁明显变厚,平滑肌细胞排列紊乱,可见大量内皮细胞增生、脱落及炎性细胞浸润,且出现明显动脉硬化斑块,与M组相比,T、G两组血管形态有所改善,动脉硬化斑块明显减少,且G组比T组改善明显;与N组比较,M组血清中内皮素(ET)-1、肝细胞生长因子(HGF)显著升高,NO显著降低(P<0.05);与M组比较,T、G两组血清中ET-1、HGF明显降低,NO显著升高,且G组与T组相比差异显著(P<0.05);与N组比较,M组血清中超氧化物歧化酶(SOD)含量显著降低,丙二醛(MDA)含量显著升高(P<0.05);与M组比较,T、G两组SOD含量显著升高,MDA含量显著降低,且G组比T组变化显著(P<0.05);与N组比较,M组血管组织中S100B、细胞外信号调节激酶(ERK)、核因子(NF)-κB蛋白表达明显升高(P<0.05);与M组比较,T、G两组血管组织中S100B、ERK、NF-κB蛋白表达均明显降低,且G组比T组降低显著(P<0.05),而P组与G组相比无明显差异(P>0.05),O组比P组降低明显(P<0.05)。结论 人参黄芩配伍可显著改善下肢动脉硬化闭塞症大鼠内皮细胞功能及氧化应激,其机制可能与抑制S100B信号通路有关。

单纯疱疹病毒感染后脑脊液S100B、Cys-C、MMP-9水平对自身免疫性脑炎的预测价值

目的:探究单纯疱疹病毒(HSV)感染后脑脊液(CSF)中S100B、Cys-C、MMP-9水平对自身免疫性脑炎(AE)的预测价值。方法:选取2016年1月至2021年3月河北中石油中心医院收治的200例HSV感染患者为研究对象,根据是否继发AE分为研究组(继发AE,35例)和对照组(未继发AE,165例)。多因素Logistic回归分析HSV感染患者继发AE的独立影响因素。Spearman法分析脑脊液中Cys-C、MMP-9与S100B水平的相关性。受试者工作特征(ROC)曲线分析S100B、Cys-C、MMP-9对AE的预测价值。构建风险预测模型并进行评价。结果:多因素Logistic回归分析显示,MRI异常、脑脊液S100B、MMP-9升高、EEG异常是HSV感染患者继发AE的独立危险因素,脑脊液Cys-C是其保护因素(P<0.05)。Spearman分析显示,HSV感染患者Cys-C浓度与S100B水平呈负相关(r=-0.83,P<0.05),MMP-9浓度与S100B水平呈正相关(r=0.88,P<0.05)。构建的联合预测因子pre1诊断HSV患者继发AE的AUC明显大于S100B、Cys-C、MMP-9单独预测的AUC(0.876 vs 0.827、0.787、0.750)。构建的风险预测模型具有良好的区分度和一致性。结论:脑脊液中S100B、Cys-C、MMP-9水平均可对HSV感染患者诱发AE的可能性进行有效预测,且三项指标联合预测价值最大,其次是S100B蛋白、Cys-C、MMP-9。

通窍化栓汤联合长春西汀及阿司匹林治疗急性脑梗死的疗效及对血液流变学和血清S100B、MMP-9的影响

【目的】探讨通窍化栓汤(由大血藤、见血飞和血三七等中药组成)联合长春西汀及阿司匹林治疗急性脑梗死的疗效及对血液流变学、血清钙结合蛋白(S100B)和基质金属蛋白酶9(MMP-9)水平的影响。【方法】将116例急性脑梗死气虚血瘀证患者随机分为对照组和观察组,每组各58例。2组患者入院后均给予对症及维持生命体征平稳、控制血压、降颅内压等常规治疗。在此基础上,对照组患者给予阿司匹林肠溶片联合长春西汀治疗,观察组在对照组的基础上给予通窍化栓汤治疗,疗程为14 d。观察2组患者治疗前后中医证候积分、美国国立卫生研究院卒中量表(NIHSS)评分、日常生活活动能力(ADL)评分、血液流变学指标、血小板功能指标和血清S100B、MMP-9水平的变化情况,并评价2组患者的临床疗效。【结果】(1)临床疗效方面,治疗14 d后,观察组的总有效率为91.38%(53/58),对照组为77.59%(45/58),组间比较(χ2检验),观察组的疗效明显优于对照组(P<0.05)。(2)量表评分方面,治疗后,2组患者的中医证候积分、NIHSS评分均较治疗前明显降低(P<0.05或P<0.01),ADL评分均较治疗前明显升高(P<0.05),且观察组对中医证候积分、NIHSS评分的降低幅度和对ADL评分的升高幅度均明显优于对照组(P<0.01)。(3)血液流变学指标方面,治疗后,2组患者的全血高切黏度、全血低切黏度、血浆黏度和纤维蛋白原水平均较治疗前明显降低(P<0.05),且观察组的降低幅度均明显优于对照组(P<0.05或P<0.01)。(4)血小板功能指标方面,治疗后,2组患者的血小板聚集率(PAgT)、血小板黏附率(PAdT)水平均较治疗前明显降低(P<0.05),且观察组的降低幅度均明显优于对照组(P<0.01)。(5)血清S100B和MMP-9水平方面,治疗后,2组患者的血清S100B和MMP-9水平均较治疗前明显降低(P<0.05),且观察组的降低幅度均明显优于对照组(P<0.01)。【结论】通窍化栓汤联合长春西汀和阿司匹林治疗急性脑梗死效果显著,可有效改善患者血液流变学指标和血小板功能,降低血清S100B和MMP-9表达水平,提高患者日常生活能力。

血清S100B蛋白联合子宫动脉阻力指数、子宫动脉搏动指数预测子痫前期的价值

目的探讨妊娠妇女血清中S100B蛋白浓度、子宫动脉搏动指数(uterine artery pulsation index,UtA-PI)、子宫动脉阻力指数(uterine artery resistance index,UtA-RI)三者单独及联合预测子痫前期的价值。方法选择2018年9月至2020年1月在青岛市市立医院产科建档产检的孕妇,共计1000例。在13~16周采用ELISA法检测血清中S100B蛋白浓度;在22~24周采用彩色多普勒超声检测孕妇的UtA-PI、UtA-RI。根据妊娠结局进行分组,子痫前期患者设为病例组(n=37),按照1∶5的比例,随机选择无妊娠合并症及并发症的孕妇作为对照组(n=185),分别评价三者单独预测子痫前期及联合预测子痫前期的效能。结果(1)血清中S100B蛋白浓度,病例组为(0.30±0.15)ng/mL,对照组为(0.10±0.04)ng/mL,病例组明显高于对照组(P<0.05)。(2)妊娠22~24周UtA-PI、UtA-RI,病例组为(0.77±0.13)、(0.38±0.10),对照组为(0.58±0.05)、(0.15±0.07),病例组均明显高于对照组(P<0.05)。(3)通过Logistic回归分析,三者均与子痫前期的发生呈正相关。(4)通过受试者工作特征曲线(ROC)分析预测效能,S100B、UtA-PI、UtA-RI单独及联合预测子痫前期,ROC曲线下面积分别为0.669(P=0.035,95%CI:0.576~0.782)、0.673(P=0.042,95%CI:0.793~0.978)、0.655(P=0.021,95%CI:0.812~0.996)、0.870(P=0,95%CI:0.626~0.936)。结论(1)孕妇血清中S100B蛋白及UtA-PI、UtA-RI均有预测子痫前期的效能,其中UtA-PI预测效能最高。(2)三者联合预测子痫前期效能最高。

中重度颅脑创伤患者血清STC1 S100B和NETRIN-1的表达及对预后的预测价值

目的探讨斯钙素抗体-1(STC1)、S100钙结合蛋白B(S100B)、轴突生长诱向因子-1(NETRIN-1)在中重度创伤性颅脑损伤(TBI)术后患者血清中的表达水平及预测预后的价值。方法收集74例TBI患者及40名健康者的血清样本,使用q RT-PCR检测健康者与TBI患者术前及术后第1天、第3天、第5天、第7天的血清STC1、S100B、NETRIN-1表达水平。收集TBI患者的一般临床资料,使用扩展版格拉斯哥结局量表(EGOS)评估患者预后,根据EGOS评分将患者分为预后良好组(EGOS≥5分,n=40)及预后不良组(EGOS<5分,n=34)。分析TBI患者术后血清STC1、S100B、NETRIN-1表达水平与预后的关系。采用受试者工作特征(ROC)曲线分析STC1、S100B、NETRIN-1表达水平对患者预后的预测价值,多因素Logistic分析评估引起TBI患者预后不良的因素。结果q RT-PCR分析显示,与健康者相比,TBI患者术前血清STC1、S100B水平升高,NETRIN-1水平降低,术后血清STC1、S100B水平降低,NETRIN-1水平升高(P<0.05)。TBI患者术后第1、3、5、7天血清STC1、S100B水平逐渐降低,NETRIN-1水平逐渐升高,术后第5天最显著(P<0.05)。与术后第5天预后良好组患者相比,预后不良组患者血清STC1、S100B水平显著升高,NETRIN-1水平显著降低(P<0.05)。皮尔逊相关性分析显示术后第5天TBI患者血清STC1、S100B水平与APACHEⅡ评分呈正比,NETRIN-1水平与APACHEⅡ评分呈反比(P<0.05)。ROC曲线分析发现术后第5天血清STC1、S100B、NETRIN-1水平对TBI患者预后具有预测价值,多因素Logistic回归分析显示仅STC1水平与患者预后相关(P<0.05)。结论STC1、S100B、NETRIN-1在TBI患者血清中表达水平异常,对TBI患者预后分析具有较高价值。

S100B时间分辨荧光免疫检测试剂盒的制备及性能评价

目的:制备一种快捷、准确、定量检测血清中S100B蛋白浓度的时间分辨荧光免疫检测试剂盒,并对其进行性能评价。方法:使用时间分辨荧光微球标记的抗S100B多克隆抗体及兔IgG抗体、标记垫、样品垫、S100B硝酸纤维素膜板、吸水纸制备试纸条,组装卡壳得到S100B时间分辨荧光免疫层析试剂盒。通过标准曲线、准确度、最低检测限、线性区间、特异度、重复性、稳定性等检测对该试剂盒进行性能评估。采用该试剂盒对某地区199例健康者血清及血浆样本的参考区间进行研究,并采用同步盲法测试该试剂盒与罗氏Elecsys S100检测试剂盒的临床应用性能,评估2种试剂盒对于142例样本检测结果的一致性。结果:该试剂盒所得标准曲线方程为y=(1.13302+1.75224)/[1+(x/1.08220)×(-0.60352)]-1.75224,R2=0.99908,线性范围为[0.05,30]ng/mL。该试剂盒可满足准确度相对偏差在±15%内、最低检测限≤0.05 ng/mL、特异度相对偏差在±15%内、批内差和批间差的变异系数均<15%的产品设计要求。稳定性检测结果标明该试剂盒可在2~30℃条件下有效保存12个月。同时,通过该试剂盒测得血清及血浆样本参考区间均<0.3 ng/mL。临床验证结果表明该试剂盒与罗氏Elecsys S100检测试剂盒的测定结果具有高度一致性(Kappa=0.9061>0.80),符合标准。结论:该试剂盒可快捷、准确、定量检测血清中S100B蛋白浓度,为神经类疾病、自身免疫病性疾病、脑血管疾病等的诊断与治疗提供了参考。

老年脊柱骨折伴脊髓损伤患者早期血清pNF-H、NSE、S100B、C反应蛋白动态变化及意义

目的探讨老年脊柱骨折伴脊髓损伤患者早期血清神经丝蛋白H磷酸化亚型(pNF-H)、神经元特异性烯醇化酶(NSE)、S100B钙结合蛋白(S100B)、C反应蛋白动态变化特点及意义。方法老年脊柱骨折患者120例根据脊髓损伤神经功能评估结果分为脊髓未损伤组83例,脊髓不完全损伤组24例,脊髓完全损伤组13例。均行前路减压内固定术治疗,分别于脊柱骨折后12、24 h、7、14 d抽取空腹外周静脉血5 ml,酶联免疫吸附试验检测血清pNF-H、NSE、S100B、C反应蛋白水平。结果脊髓完全损伤组和脊髓不完全损伤组脊髓损伤后12、24 h、7 d血清pNF-H、NSE、S100B、C反应蛋白浓度逐渐升高,脊髓损伤后14 d下降;脊髓未损伤组脊髓损伤后12、24 h、7、14 d血清pNF-H、NSE、S100B、C反应蛋白浓度无明显变化。脊髓完全损伤组脊髓损伤后12、24 h、7、14 d血清pNF-H、NSE、S100B、C反应蛋白浓度明显高于脊髓不完全损伤组和脊髓未损伤组,脊髓不完全损伤组明显高于脊髓未损伤组(P<0.05)。受试者工作特征(ROC)曲线分析显示,血清pNF-H、NSE、S100B、C反应蛋白对老年脊柱骨折伴脊髓损伤均具有较高的诊断价值,其中血清pNF-H、NSE、S100B、C反应蛋白联合检测的诊断价值最高[曲线下面积(AUC)=0.857],灵敏度87.348%、特异度83.581%,高于各指标单独检测。结论pNF-H、NSE、S100B、C反应蛋白4项血清学指标联合检测在脊柱骨折伴脊髓损伤早期诊断和病情严重程度评估中具有较高的应用价值。

脑损伤患者S100B蛋白截断值的探究

目的探讨脑损伤患者S100钙结合蛋白B(S100B)蛋白截断值及价值。方法选取2021年6月—2022年12月在潍坊市中医院住院收治的脑损伤患者181例为观察组,根据患者疾病类型分为创伤性脑损伤组(53例)、急性脑梗死组(62例)和出血性脑卒中组(66例);创伤性脑损伤患者,根据病情严重程度分为轻型组(21例)、中型组(17例)、重型组(10例)及特重型组(5例)。根据格拉斯哥结局量表评分分为存活组(144例)和死亡组(37例);选择该时间段内健康体检者50名作为对照组;采用金磁微粒免疫层析法测定各组血清中S100B蛋白水平;绘制ROC曲线,分析S100B蛋白在脑损伤患者中的截断值,以试剂盒原参考范围作为参考,完成一致性分析。结果观察组S100B蛋白水平高于对照组(P<0.05);创伤组、梗死组和出血组不同时间点S100B蛋白水平差异有统计学意义(P<0.05);存活组不同时间点S100B蛋白水平低于死亡组(P<0.05);创伤组不同亚型分组下,随着时间的延长血清中S100B蛋白水平表现为先上升后下降趋势,并于48 h达到峰值。S100B蛋白水平不同时间点特重型组>重型组>中型组>轻型组(P<0.05);血清S100B蛋白的ROC曲线下面积为0.901,截断值为90.80 pg/mL,灵敏度为0.65,特异度为0.98(P<0.05);以试剂盒原参考范围作为参考,该截断值Kappa值为0.863。结论脑损伤患者S100B蛋白水平较高,其表达水平能反映患者预后;以试剂盒原参考范围作为参考进行诊断时漏诊率较高,通过确定脑损伤患者S100B蛋白截断值能缩小正常人群参考范围。

钙结合蛋白S100A4通过TLR4/NF-κB信号通路调控胶质瘤细胞增殖、存活及迁移功能

目的:探索外源性钙结合蛋白S100A4对胶质瘤细胞增殖、存活及迁移功能的影响及机制。方法:利用UCSC数据库下载泛癌数据集,进行S100A4在泛癌中的表达及预后分析;从CGGA数据库中下载胶质瘤患者的转录组数据和临床数据,利用R软件进行分析S100A4表达在胶质瘤患者中的预后与进展;利用在线分析工具GEPIA与STRING进行胶质瘤患者的S100A4蛋白质网络互作分析。体外培养人胶质瘤细胞系(U87与U251),实验分为3组:PBS组、S100A4组、S100A4+TAK242组[瑞沙托维(TAK242)为Toll-样受体4(TLR4)特异性抑制剂]。流式细胞术检测胶质瘤细胞的增殖与凋亡;细胞划痕实验、Transwell实验及克隆形成实验检测U87与U251细胞的迁移及增殖能力;Western blot检测TLR4蛋白、NF-κB相关信号分子蛋白水平。结果:生物信息学结果显示,S100A4在多种肿瘤中显著上调(P<0.05),包括:胶质母细胞瘤(GBM)、低级胶质瘤(LGG)、胃癌(STAD)、肝细胞肝癌(LIHC)等,其中在GBM和LGG中预后较差。与低表达S1004的胶质瘤患者相比,高表达S100A4的胶质瘤患者生存期更短,WHO分级程度更高。此外,胶质瘤患者S100A4蛋白可能与膜联蛋白A2(ANXA2)、TLR4和晚期糖基化终末产物特异性受体(AGER)蛋白存在相互作用。细胞实验中,与PBS组相比,外源性S100A4处理后,胶质瘤U87和U251细胞增殖、迁移能力增强,TLR4、p-ERK1/2、p-p38、p-p65蛋白水平显著上调(P<0.05)。与S100A4组相比,S100A4+TAK242组胶质瘤细胞增殖、迁移能力减弱,TLR4、p-ERK1/2、p-p38、p-p65蛋白水平显著下调(P<0.05)。结论:S100A4可能通过TLR-4/NF-κB信号通路调控胶质瘤细胞增殖、迁移及存活功能。

胎膜早破宫内感染产妇脐血和羊水中miR-182、TNF-α、S100B预测早产儿脑损伤价值

目的:探究胎膜早破宫内感染产妇脐血和羊水中微小核糖核酸182(miR-182)、肿瘤坏死因子-α(TNF-α)及S100钙结合蛋白B(S100B)预测早产儿脑损伤的临床价值。方法:选取2021年6月-2023年6月在本院分娩的104例胎膜早破宫内感染产妇临床资料,分娩的早产儿胎龄均<34周,行头部影像学检查,根据是否发生脑损伤将产妇分为脑损伤组(n=36)与非脑脑损伤组(n=68)。检测并比较两组脐血和羊水中miR-182、TNF-α、S100B蛋白水平,采用受试者工作特征(ROC)曲线评价胎膜早破宫内感染产妇脐血和羊水miR-182、TNF-α及S100B蛋白对早产儿脑损伤的预测价值。结果:脑损伤组脐血miR-182、TNF-α、S100B蛋白水平均高于非脑损伤组,羊水miR-182、TNF-α均高于非脑损伤组(均P<0.05),羊水中S100B蛋白水平两组无差异(P>0.05)。ROC曲线分析,脐血miR-182、TNF-α、S100B蛋白预测早产儿脑损伤的曲线下面积(AUC)分别为0.816、0.748、0.697,灵敏度分别为72.2%、66.7%、55.6%,特异度分别为83.8%、77.9%、88.2%;羊水miR-182、TNF-α、S100B蛋白预测早产儿脑损伤的AUC分别为0.713、0.689、0.594,灵敏度分别为63.9%、55.6%、30.6%,特异度分别为86.8%、85.3%、86.8%。结论:胎膜早破宫内感染产妇脐血和羊水中miR-182、TNF-α、S100B蛋白预测其早产儿脑损伤均有一定价值。

脑脊液中TXB2、S100B水平与高血压脑出血患者预后的相关性

目的探究脑脊液中血栓素B2(thromboxane B2,TXB2)、S100钙结合蛋白B(S100 calcium-binding protein B,S100B)水平与高血压脑出血患者预后的相关性。方法选取2020年5月至2023年5月西安市长安医院急诊收治的高血压脑出血患者96例,均行微创血肿清除术治疗,收集所有患者的病历资料,检测患者术后24 h脑脊液中的TXB2、S100B水平。依据患者术后28 d预后分为预后良好组和预后不良组。分析高血压脑出血预后的影响因素,评价脑脊液中TXB2、S100B水平对高血压脑出血患者预后的预测效能。采用χ^(2)检验、独立样本t检验,影响因素的分析采用多因素logistic逐步回归模型。结果术后28 d,96例高血压脑出血患者中预后良好68例(70.83%),预后不良28例(29.17%)。两组性别、年龄、体重指数等一般资料比较,差异均无统计学意义(均P>0.05);预后良好组美国国立卫生研究院卒中量表(NIHSS)评分、中线移位占比及脑脊液TXB2、S100B水平均低于预后不良组[(15.34±2.61)分比(20.18±3.32)分、19.12%(13/68)比39.29%(11/28)、(156.04±17.31)ng/L比(190.35±18.29)ng/L、(1.72±0.34)μg/L比(1.93±0.47)μg/L],差异均有统计学意义(均P<0.05)。NIHSS评分(OR=3.691,95%CI 1.262~10.799)、中线移位(OR=3.425,95%CI 1.171~10.019)、脑脊液TXB2(OR=5.675,95%CI 1.939~16.602)及S100B(OR=4.486,95%CI 1.533~13.125)是高血压脑出血预后的危险因素(均P<0.05)。脑脊液中TXB2、S100B单一及联合预测高血压脑出血患者预后的灵敏度分别为0.764、0.727、0.799,特异度分别为0.641、0.703、0.782,曲线下面积分别为0.731、0.705、0.823。结论脑脊液中TXB2、S100B水平的变化与高血压脑出血患者预后有关,且两者联合检测对高血压脑出血患者预后的预测效能良好。

血清GDNF、S100B、维生素D水平对产后抑郁症的预测价值分析

目的:探讨血清胶质细胞源性神经营养因子(GDNF)、S100钙结合蛋白B(S100B)、维生素D水平联合检测对剖宫产产妇发生产后抑郁的预测价值。方法:选取2021年9月—2023年9月某院产科孕39周以上待产孕妇104例为研究对象,均行剖宫产,根据爱丁堡抑郁量表(EPDS)评估产后抑郁情况,将发生产后抑郁产妇纳入观察组(18例),未发生产后抑郁产妇纳入对照组(86例)。比较2组产前、产后3 d EPDS评分及血清GDNF、S100B、维生素D水平,分析血清各指标水平与EPDS评分之间的相关性,分析血清各指标联合检测对产后抑郁的预测价值。结果:产后3 d,观察组EPDS评分[(18.93±2.24)分]高于对照组[(7.04±0.96)分](P<0.05);产后3 d,观察组血清GDNF、维生素D水平[(5.63±1.28)pg/mL、(22.85±3.26)ng/mL]低于对照组[(12.55±3.07)pg/mL、(32.19±4.02)ng/mL],血清S100B水平[(63.29±5.18)μg/mL]高于对照组[(42.67±3.49)μg/mL],差异均有统计学意义(P<0.05)。产后3 d,血清GDNF、维生素D水平与EPDS评分呈负相关(r=-0.624、-0.549,P均<0.05),S100B水平与EPDS评分呈正相关(r=0.573,P<0.05),且各指标联合预测产后抑郁的AUC为0.938(95%CI:0.873~0.976),最佳诊断敏感度为88.89%,特异度为87.21%,约登指数为0.761。结论:剖宫产产后抑郁患者血清中GDNF、维生素D表达下调,S100B表达上调,各指标水平与EPDS评分均具有一定相关性,联合检测可作为临床评估产后抑郁情况的辅助指标。

S100b联合CRP在诊断早产儿脑损伤中的临床价值

目的探讨S100b联合CRP在诊断早产儿脑损伤(Brain injury in premature infants,BIPI)中的临床效能。方法选择2022年1月—2024年1月于本院儿科确诊的125例BIPI患儿作为BIPI组,另选择同期收治的85例非BIPI早产儿作为对照组。根据BIPI患儿病情严重程度分为轻度BIPI组和重度BIPI组两组亚组。收集所有研究对象的临床资料并检测血清中S100b联合CRP表达水平。Logistic回归分析发生BIPI的危险因素,S100b联合CRP在诊断BIPI的临床效能采用ROC曲线分析。结果对照组、轻度BIPI组和重度BIPI组三组间S100b、CRP表达水平存在统计学差异(P<0.05)。与对照组相比,轻度和重度BIPI组S100b、CRP表达水平均明显升高(P<0.05);与轻度BIPI组相比,重度BIPI组S100b、CRP表达水平均明显升高(P<0.05)。与对照组相比,宫内窘迫、出生后窒息、有创机械通气、新生儿呼吸窘迫综合征发生率及血清中S100b、CRP表达水平在BIPI组中明显升高(P<0.05)。Logistic回归分析结果显示,有创机械通气(OR=1.432)、新生儿呼吸窘迫综合征(OR=2.543)、S100b(OR=3.782)和CRP表达(OR=3.449)是发生BIPI的危险因素。S100b及CRP在诊断BIPI的曲线下面积分别为0.895和0.812,S100b联合CRP在诊断BIPI的曲线下面积为0.931,诊断敏感度和特异度分别为97.43%和92.25%。结论BIPI患儿外周血中S100b和CRP表达水平显著升高,S100b联合CRP在诊断BIPI中具有显著的临床价值。

S100B protein in tissue development,repair and regeneration

The Ca 2+-binding protein of the EF-hand type,S100B,exerts both intracellular and extracellular regulatory activities.As an intracellular regulator,S100B is involved in the regulation of energy metabolism,transcription,protein phosphorylation,cell proliferation,survival,differentiation and motility,and Ca 2+ homeostasis,by interacting with a wide array of proteins(i.e.,enzymes,enzyme substrates,cytoskeletal subunits,scaffold/adaptor proteins,transcription factors,ubiquitin E3 ligases,ion channels) in a restricted number of cell types.As an extracellular signal,S100B engages the pattern recognition receptor,receptor for advanced glycation end-products(RAGE),on immune cells as well as on neuronal,astrocytic and microglial cells,vascular smooth muscle cells,skeletal myoblasts and cardiomyocytes.However,RAGE may not be the sole receptor activated by S100B,the protein being able to enhance bFGF-FGFR1 signaling by interacting with FGFR1-bound bFGF in particular cell types.Moreover,extracellular effects of S100B vary depending on its local concentration.Increasing evidence suggests that at the concentration found in extracellular fluids in normal physiological conditions and locally upon acute tissue injury,which is up to a few nM levels,S100B exerts trophic effects in the central and peripheral nervous system and in skeletal muscle tissue thus participating in tissue homeostasis.The present commentary summarizes results implicating intracellular and extracellular S100B in tissue development,repair and regeneration.

S100B protein in serum is elevated after global cerebral ischemic injury

BACKGROUND:S100B protein in patients with cardiac arrest,hemorrhagic shock and other causes of global cerebral ischemic injury will be dramatically increased.Ischemic brain injury may elevate the level of serum S100 B protein and the severity of brain damage.METHODS:This article is a critical and descriptive review on S100 B protein in serum after ischemic brain injury.We searched Pubmed database with key words or terms such as "S100B protein", "cardiac arrest", "hemorrhagic shock" and "ischemia reperfusion injury" appeared in the last five years.RESULTS:S100B protein in patients with cardiac arrest,hemorrhagic shock and other causes of ischemic brain injury will be dramatically increased.Ischemic brain injury elevated the level of serum S100 B protein,and the severity of brain damage.CONCLUSION:The level of S100 B protein in serum is elevated after ischemic brain injury,but its mechanism is unclear.

S100 calcium binding protein A6 and associated long noncoding ribonucleic acids as biomarkers in the diagnosis and staging of primary biliary cholangitis

BACKGROUND Primary biliary cholangitis(PBC)is a chronic and slowly progressing cholestatic disease,which causes damage to the small intrahepatic bile duct by immunoregulation,and may lead to cholestasis,liver fibrosis,cirrhosis and,eventually,liver failure.AIM To explore the potential diagnosis and staging value of plasma S100 calcium binding protein A6(S100A6)messenger ribonucleic acid(mRNA),LINC00312,LINC00472,and LINC01257 in primary biliary cholangitis.METHODS A total of 145 PBC patients and 110 healthy controls(HCs)were enrolled.Among them,80 PBC patients and 60 HCs were used as the training set,and 65 PBC patients and 50 HCs were used as the validation set.The relative expression levels of plasma S100A6 mRNA,long noncoding ribonucleic acids LINC00312,LINC00472 and LINC01257 were analyzed using quantitative reverse transcription-polymerase chain reaction.The bile duct ligation(BDL)mouse model was used to simulate PBC.Then double immunofluorescence was conducted to verify the overexpression of S100A6 protein in intrahepatic bile duct cells of BDL mice.Human intrahepatic biliary epithelial cells were treated with glycochenodeoxycholate to simulate the cholestatic environment of intrahepatic biliary epithelial cells in PBC.RESULTS The expression of S100A6 protein in intrahepatic bile duct cells was up-regulated in the BDL mouse model compared with sham mice.The relative expression levels of plasma S100A6 mRNA,log10 LINC00472 and LINC01257 were upregulated while LINC00312 was down-regulated in plasma of PBC patients compared with HCs(3.01±1.04 vs 2.09±0.87,P<0.0001;2.46±1.03 vs 1.77±0.84,P<0.0001;3.49±1.64 vs 2.37±0.96,P<0.0001;1.70±0.33 vs 2.07±0.53,P<0.0001,respectively).The relative expression levels of S100A6 mRNA,LINC00472 and LINC01257 were up-regulated and LINC00312 was down-regulated in human intrahepatic biliary epithelial cells treated with glycochenodeoxycholate compared with control(2.97±0.43 vs 1.09±0.08,P=0.0018;2.70±0.26 vs 1.10±0.10,P=0.0006;2.23±0.21 vs 1.10±0.10,P=0.0011;1.20±0.04 vs 3.03±0.15,P<0.0001,respectively).The mean expression of S100A6 in the advanced stage(III and IV)of PBC was up-regulated compared to that in HCs and the early stage(II)(3.38±0.71 vs 2.09±0.87,P<0.0001;3.38±0.71 vs 2.57±1.21,P=0.0003,respectively);and in the early stage(II),it was higher than that in HCs(2.57±1.21 vs 2.09±0.87,P=0.03).The mean expression of LINC00312 in the advanced stage was lower than that in the early stage and HCs(1.39±0.29 vs 1.56±0.33,P=0.01;1.39±0.29 vs 2.07±0.53,P<0.0001,respectively);in addition,the mean expression of LINC00312 in the early stage was lower than that in HCs(1.56±0.33 vs 2.07±0.53,P<0.0001).The mean expression of log10 LINC00472 in the advanced stage was higher than those in the early stage and HCs(2.99±0.87 vs 1.81±0.83,P<0.0001;2.99±0.87 vs 1.77±0.84,P<0.0001,respectively).The mean expression of LINC01257 in both the early stage and advanced stage were up-regulated compared with HCs(3.88±1.55 vs 2.37±0.96,P<0.0001;3.57±1.79 vs 2.37±0.96,P<0.0001,respectively).The areas under the curves(AUC)for S100A6,LINC00312,log10 LINC00472 and LINC01257 in PBC diagnosis were 0.759,0.7292,0.6942 and 0.7158,respectively.Furthermore,the AUC for these four genes in PBC staging were 0.666,0.661,0.839 and 0.5549,respectively.The expression levels of S100A6 mRNA,log10 LINC00472,and LINC01257 in plasma of PBC patients were decreased(2.35±1.02 vs 3.06±1.04,P=0.0018;1.99±0.83 vs 2.33±0.96,P=0.036;2.84±0.92 vs 3.69±1.54,P=0.0006),and the expression level of LINC00312 was increased(1.95±0.35 vs 1.73±0.32,P=0.0007)after treatment compared with before treatment using the paired t-test.Relative expression of S100A6 mRNA was positively correlated with log10 LINC00472(r=0.683,P<0.0001);serum level of collagen type IV was positively correlated with the relative expression of log10 LINC00472(r=0.482,P<0.0001);relative expression of S100A6 mRNA was positively correlated with the serum level of collagen type IV(r=0.732,P<0.0001).The AUC for the four biomarkers obtained in the validation set were close to the training set.CONCLUSION These four genes may potentially act as novel biomarkers for the diagnosis of PBC.Moreover,LINC00472 acts as a potential biomarker for staging in PBC.

S100 protein expression during induced Schwann cell-like cell differentiation of rat bone marrow mesenchymal cells in vitro

BACKGROUND： S100 protein can promote axonal growth. Therefore, transplantation of induced bone marrow-derived mesenchymal stem cells （MSCs） that can secrete S100 may provide a beneficial microenvironment for neural regeneration. OBJECTIVE： To explore the changes in S100 expression during rat MSCs differentiation into Schwann ceils in vitro. DESIGN, TIME AND SETTING： This cytology experiment was performed at the Jiangsu Key Laboratory of Neuroregeneration, Nantong University in China, from January 2006 to May 2007. MATERIALS： The rabbit anti-S100 polyclonal antibody was purchased from Dako, Denmark; the mouse anti-rat S100 monoclonal antibody was purchased from Sigma, USA. METHODS： MSCs were cultured from adult Sprague-Dawley rat femur and tibia. Cell proliferation was determined by the MTT method and CD markers, and cell cycle was measured by flow cytometry. MSCs were induced to differentiate into SC cells. SC cells were stained for S100 protein, glial fibrillary acidic protein, and low-affinity nerve growth factor receptor. S100 protein and mRNA levels were evaluated by flow cytometry, Western blot, and reverse transcription-polymerase chain reaction. MAIN OUTCOME MEASURES： S100 protein and mRNA expression. RESULTS： MSCs exhibited high amplification potential over eight passages. Prior to induction, the majority of MSCs were at the G0/G1 phase of the cell cycle. After induction, MSCs displayed morphology changes similar to Schwann cells. Moreover, induction increased S100 mRNA levels. Immunofluorescence showed that MSCs expressed S100 protein, glial fibrillary acidic protein, and low-affinity nerve growth factor receptor at 7 days of induction. Induction also increased S100 protein levels compared with untreated MSCs. CONCLUSION： MSCs are capable of differentiating into Schwann cells-like cells under conditional induction in vitro, with increasing S100 mRNA and protein expression.