Expressions and clinical significances of mannose-binding lectin(MBL) and MBL-associated serine protease 2(MASP-2) in patients with thyroid neoplasm

Objective： The aim of the study was to detect the levels of mannose-binding lectin （MBL）, MBL-associated serine protease 2 （MASP-2） and explore the clinical significances of them in patients with primary thyroid neoplasms. Methods： By using ELISA method, we detected the serum levels of MBL and MASP-2 in 26 patients with papillary thyroid carcinoma （PTC）, 30 patients with thyroid adenoma （TA） and 26 healthy people, respectively. Results： Serum MBL level was （565.23 ± 76.70） μg/L in PTCs higher than （324.267 ±24.74） μg/L in TAs, and （152.69± 16.95） IJg/L in healthy of controlling group. There was statistical significance between PTC and TA （P 〈 0.05）, however there was no difference between TA and healthy （P 〉 0.05）. Serum MASP-2 level was （726.153± 78.88） pg/L in PTCs higher than （379.266 ± 30.26） μg/L in TAs, and （203.846 ± 29.09） μg/L in healthy. Serum MASP-2 level was higher in PTCs than TAs, and the difference had statistical significance （P 〈 0.01）. But no difference was observed between in TAs and healthy. Conclusion： These findings might reflect inflammatory processes induced by defense mechanisms, in response to the development of the turnout. MBL may also be involved in the elimination of possible tumourigenic pathogens.

Mannose-binding Lectin Two Gene Polymorphisms and Tuberculosis Susceptibility in Chinese Population: A Meta-analysis

Numerous studies have been done to explore the association between mannose-binding lectin two （MBL2） gene polymorphisms and the risk of tuberculosis （TB）. However, the results are inconsistent. We performed a meta-aualysis to investigate whether polymorphisms in the MBL2 gene were associated with TB risk. Databases including PubMed, Medline, Chinese Biomedicine Database, China National Knowledge Infrastructure, Wanfang Database, and Weipu Database were searched to find relevant articles published up to 2 October, 2012. Odds ratio （OR） with 95% confidence interval （CI） was used to evaluate the strength of association. All statistical tests were performed by using Revman 5.1 software and STATA 11.0 software. Six case-control studies including 1106 cases and 1190 controls were accepted in the meta-analysis. The results indicated that individuals carrying the MBL2 codon 54 B allele may have an increased risk of TB as compared with AA homozygotes （BB＋AB vs. AA： OR=1.52, 95% CI： 1.22-1.88）, whereas MBL2 ＋4 P/Q was possibly not associated with TB susceptibility in Chinese population.

Mannose-binding lectin and maladies of the bowel and liver

Mannose-binding lectin (MBL) is a pattern-recognition molecule that binds to characteristic carbohydrate mo-tifs present on the surface of many different pathogens. MBL binding stimulates the immune system via the lectin pathway of complement activation. In certain clinical situations, often characterized by pre-existing immune compromise, MBL deficiency increases the risk of infec-tious and other disease-specific complications. Many of the key pathogenic processes inherent to common gastroenterological diseases, such as infection, immuno-logical damage, and carcinogenesis, have been linked to MBL. This editorial reviews the biology of MBL, outlines key disease associations to document the breadth of influence of MBL, and finally, highlights the relevance of MBL to both gastroenterological health and disease.

Mannose-binding lectin 2 rs11003123 polymorphism is associated with the development of hepatocellular carcinoma in patients with hepatitis B-related cirrhosis in the Chinese population

BACKGROUND： Mannose-binding lectin 2 （MBL2） plays a key role in the host immune response, but whether it is associ- ated with hepatocellular carcinoma （HCC） is not dear. The present study aimed to identify the association between MBL2 gene polymorphisms and HCC in patients with hepatitis B virus （I-IBV）-related cirrhosis in the Chinese population.

Early expression of mannose-binding lectin 2 during Aspergillus fumigatus infection in human corneal epithelial cells

AIM: To evaluate the early expression of mannose-binding lectin 2(MBL2) in human corneal epithelial cells(HCECs) infected by Aspergillus fumigatus(AF).METHODS: HCECs cultured in vitro with AF antigens and sampled at 0, 0.5, 1, 2, 4, 6 and 8h. The expression of MBL2 m RNA was evaluated by semiquantitative reverse transcription-polymerase chain reaction(RT-PCR). The expression of MBL2 protein in supernatant fluid was shown by enzyme linked immunosorbent assay(ELISA). MBL2 protein in HCECs was detected by immunocytochemistry at 0 and 24 h.RESULTS: MBL2 m RNA and protein are expressed in normal HCECs. The expression of MBL2 m RNA and protein in supernatant fluid begin to increase after being stimulated with AF antigens. The most significantly peak of MBL2 m RNA is in 2h. The protein of MBL2 in supernatant fluid decrease gradually after 0.5h. The protein in HCECs expression increase after stimulation of24 h.· CONCLUSION: MBL2 receptor expressed in normal HCECs in vitro. The stimulation by AF antigens can increase the early expression of it.

Dietary sugars inhibit biologic functions of the pattern recognition molecule, mannose-binding lectin

Mannose-binding lectin (MBL), a mammalian lectin, is a pattern recognition molecule of the innate immune system and recognizes carbo-hydrates that are exposed on pathogens. In this study, we observed that fructose down regu-lates MBL-mediated innate immune mechanisms against both influenza A virus (IAV) and Staphy-lococcus aureus. These mechanisms include the lectin complement pathway and coagulation enzyme-like activities on both pathogens. Fur-thermore, fructose also reduces MBL-mediated phagocytosis of S. aureus and IAV and MBL- mediated IAV infection to epithelial cells. In contrast, sucrose inhibits MBL-mediated im-mune mechanisms against S. aureus but not IAV. Together, our studies show that dietary sugars, in particular fructose, negatively regulate the innate immunity against viral and bacterial pathogens.

MBL及其补体激活的LECTIN途径

MBL是一种血清C型凝集素 ,是机体先天免疫的重要分子之一 ,本文在简要总述MBL的结构和功能的基础上 ,对MBL参与的凝集素途径进行阐述。

人CGT52TGTMBL突变体在CHO细胞中的表达及其产物分析

目的: 初步探索MBL基因CGT52TGT点突变引起调理吞噬缺损的机制。方法: 采用PCR技术, 从质粒pMBLm52中获取含CGT52TGT点突变的MBL基因, 将其插入真核表达载体pcDNA4 /HisMaxC中构建重组表达载体。经测序验证后, 电转染入CHO细胞。以800mg/LZeocin筛选转染后的CHO细胞30d; 随后的30d中, 维持Zeocin的浓度在200mg/L, 以获取稳定转染的细胞。以RT PCR分析其mRNA的表达情况。表达产物经Ni NTAagarose纯化后, 以非还原SDS PAGE和Westernblot对表达产物进行初步鉴定。结果:以PCR扩增的MBLm52基因片段长约750bp, 将其插入表达载体构建重组真核表达载体pcDNA4 /HisMaxC MBLm52, 测序验证序列正确后将其电转染入CHO细胞。从细胞培养上清中获得的纯化的表达产物, 主要为相对分子质量(Mr)约60 000的分子, 寡聚化程度明显低于重组人野生型MBL和从人血浆中分离的MBL。结论: MBL基因CGT52TGT点突变可能并不影响其表达产物向胞外分泌的过程, 但突变后产生的Cys可能形成新的二硫键, 影响MBL结构单位和/或寡聚分子的形成, 推测该突变MBL蛋白不能发挥正常的功能。

雷公藤多苷抑制糖尿病大鼠肾组织MBL及MASP2的表达并减轻肾损伤

目的研究雷公藤多苷对糖尿病大鼠肾组织甘露糖结合凝集素(MBL)及甘露聚糖结合凝集素丝氨酸肽酶2(MASP2)表达的影响,探讨雷公藤多苷对糖尿病大鼠肾脏损伤的保护机制。方法 45只雄性SD大鼠随机分为实验组(n=35)和正常对照组(n=10)。实验组喂以高糖高脂饲料6周后,腹腔注射链脲佐菌素(STZ)建立糖尿病肾病大鼠模型。实验组有33只大鼠造模成功,将33只大鼠随机分为糖尿病肾病模型组(n=16)和雷公藤多苷治疗组(n=17),治疗组以雷公藤多苷[10 mg/(kg·d)]灌胃8周。第14周末,比较模型组和治疗组24 h尿蛋白定量及血清生化指标;过碘酸希夫反应(PAS)观察肾组织形态学改变;荧光定量PCR检测肾组织MBL1、MASP2、核因子κB(NF-κB)、单核细胞趋化蛋白1(MCP-1)mRNA水平,Western blot法检测肾组织MBL-A、MASP2、NF-κB、MCP-1的蛋白水平,免疫组织化学染色检测MBL-A、MASP2蛋白在肾组织的表达和分布。结果与治疗组相比,模型组大鼠24 h尿蛋白定量、血清肌酐、尿素氮增高,肾组织MBL、MASP2、NF-κB及MCP-1表达明显增加;相关性分析显示,MBL与MASP2、NF-κB、MCP-1表达及24 h尿蛋白定量呈显著正相关。结论雷公藤多苷能抑制糖尿病模型大鼠肾组织MBL及MASP2的表达,减轻糖尿病大鼠肾损伤。

类风湿关节炎患者血清MBL、MASP-2、HsCRP与C_3水平的相关性

目的研究类风湿关节炎(RA)患者血清中甘露糖结合凝集素(MBL)/MBL相关的丝氨酸蛋白酶-2(MASP-2)、Hs CRP和C3水平的相关性。方法收集50例RA患者(活动期和非活动期各25例)和40例健康对照者空腹静脉血,用酶联免疫吸附试验和免疫比浊试验分别检测血清MBL、MASP-2、Hs CRP和C3的水平。结果 RA组活动期和非活动期患者血清中MBL水平均显著低于健康对照组(10.05±2.14 ng/m L vs 26.97±11.78 ng/m L;14.79±3.93 ng/m L vs 26.97±11.78 ng/m L,P<0.05);RA组活动期和非活动期患者血清中MASP-2水平均显著低于健康对照组(75.90±9.21 ng/m L vs 251.78±34.50 ng/m L;107.8±14.90 ng/m L vs251.78±34.50 ng/m L)(P<0.05);RA组活动期和非活动期患者血清中Hs CRP水平显著高于健康对照组(40.53±34.81 mg/L vs1.42±1.70 mg/L;2.97±2.51 mg/L vs 1.42±1.70 mg/L,P<0.05),C3水平3组无差异;双变量Pearson相关性分析,RA患者组MBL与MASP-2含量均呈显著正相关(r=0.550,P=0.001)、与Hs CRP含量呈低度负性相关(r=-0.323,P=0.022);与C3含量无相关(r=0.022,P=0.882)。RA组MASP-2与Hs CRP含量呈低度负性相关(r=-0.453,P=0.001);与C3含量无相关(r=0.049,P=0.738)。经ROC曲线分析,Hs CRP曲线下面积最大(0.844,P=0.001),MASP-2和MBL曲线下面积较小(0.025,P=0.001;0.266,P=0.001),Hs CRP(84%)对RA诊断的敏感性高于MBL(10%)、MASP-2(40%)。结论 MBL与MASP-2水平与Hs CRP呈负相关关系,RA患者关节的炎症损伤程度越重,则血清MBL与MASP-2水平越低,提示MBL与MASP-2参与RA病理损伤过程,但二者的敏感性均较低,不能做为RA诊断及疾病活动程度评价的独立指标。

MBL突变体在CHO细胞中表达及其产物分析

采用PCR技术,从质粒pMBLm54中获得含GGC54GAC点突变的甘露聚糖结合凝集素(MBL)基因,将其插入真核表达载体构建重组表达载体pcDNA4/HisMax C-MBLm54,DNA测序验证序列正确后将其电转染入CHO细胞。以Zeocin筛选并维持培养转染后CHO细胞,获得2株稳定高效表达目的蛋白的单克隆细胞株。采用Ni^(2+)-NTA agarose层析柱纯化表达产物,获得54Asp突变MBL蛋白,SDS-PAGE和Western blot分析表明,54Asp突变MBL蛋白主要为相对分子质量为60000的成分,而重组野生型MBL蛋白则主要是相对分子质量为200000和>200000的分子。配体结合试验发现,天然MBL和重组野生型MBL能与甘露聚糖结合,而54Asp则否。结果表明,54Asp突变MBL蛋白不能形成正常的MBL结构单位和寡聚体,并进而影响其配体结合活性。

人血浆中MBL-MASP复合物的纯化与分离

目的从人血浆中分离纯化甘露聚糖结合凝集素(MBL)和MBL相关丝氨酸蛋白酶(MASP)。方法用非活化Sepharose4B两步亲和层析纯化MBL-MASP复合物,再以SephacrylS-300柱凝胶过滤将MBL和MASP分离。在纯化MBL-MASP复合物的整个过程中,除凝胶过滤缓冲液外,均加入丝氨酸蛋白酶抑制剂苯甲磺酰氟(PMSF)和金属蛋白酶抑制剂1,10-邻二氮杂菲(1,10-phenanthroline),并控制温度在4 ℃。结果获得高度纯化的MBL和酶原形式的MASP。SDS-PAGE和Westernblotting表明所纯化的MBL相对分子质量为28000和32000肽链构成的功能性多聚体;配体结合测定和酵母菌凝集试验证实所纯化的MBL具有生物学活性。结论建立了一种比较简便的同时分离纯化MBL和MASP酶原的方法。

类风湿性关节炎患者血清MBL MASP-2和DKK-1水平变化与患者预后相关性

目的:研究类风湿性关节炎(RA)患者血清甘露糖结合凝集素(MBL)、MBL相关的丝氨酸蛋白酶-2(MASP-2)和Dickkopf-1蛋白(DKK-1)水平变化及其与患者预后相关性。方法:选取2017年8月至2020年8月我院194例RA患者和102例健康体检者分别为研究组和对照组,检测入院时血清MBL、MASP-2和DKK-1水平,同时根据28个关节疾病活动评分(DAS28)将患者分为轻度组83例、中度组62例和重度组49例,按指南对RA患者给予达标治疗并根据疗效将患者分为达标组129例和未达标组65例,比较各组血清MBL、MASP-2和DKK-1水平,同时分析其对DAS28评分的影响和对疗效的预测价值。结果:研究组血清MBL和MASP-2水平低于对照组,血清DKK-1水平高于对照组;轻度组、中度组和重度组血清MBL和MASP-2逐渐降低,血清DKK-1水平和DAS28评分逐渐升高;达标组血清MBL和MASP-2水平高于未达标组,血清DKK-1水平低于未达标组,差异有统计学意义(P<0.05)。多元线性回归分析显示,血清MBL和MASP-2水平为影响DAS28评分的重要因素(P<0.05)。血清MBL和MASP-2水平与RA治疗效果存在密切联系,RA治疗未达标的logistics回归模型为Y=12.573-0.722×血清MBL-0.090×血清MASP-2+0.792×血清DKK-1。血清MBL、MASP-2、DKK-1及三者联合检测预测RA疗效的AUC分别为0.896、0.825、0.693和0.958,敏感度分别为72.09%、67.44%、80.62%和89.15%,特异度分别为90.77%、81.54%、52.31%和90.77%。结论:RA患者血清MBL和MASP-2水平明显降低,血清DKK-1水平明显升高,且与病情变化密切相关,可为评估疗效和预后提供参考。

MBL调控MASP激活补体系统

甘露聚糖结合凝集素(MBL;或甘露聚糖结合蛋白,MBP)是由相同的多肽链组成的寡聚物,它通过结合细胞表面的碳水化合物能够有效地识别侵入体内的多种致病微生物,并激活补体来杀灭病原微生物。MBL能与血清中其相关蛋白酶(MASP)结合,MASP包含3个丝氨酸蛋白酶MASP-1、MASP-2、MASP-3和非酶蛋白MAp19。研究显示,MBL通过2种机理调控MASP-2的活性,在先天性免疫中具有重要的作用。本文简要综述MBL调控MASP激活补体的作用机理。

HBV慢性感染者血清中MBL、MASP和C3b水平检测的临床意义

目的研究MBL、MASP和C3b在不同感染程度的乙肝患者中的表达及其临床意义。方法乙肝患者共140例,依据血清中HBeAg和ALT的水平分为6组:A组(HBeAg阳性,ALT正常)、B组(HBeAg阴性,ALT正常)、C组(HBeAg阳性,ALT轻度/中度升高)、D组(HBeAg阳性,ALT高度/重度升高)、E组(HBeAg阴性,ALT轻度/中度升高)、F组(HBeAg阴性,ALT高度/重度升高)。采用ELISA法检测健康对照(G组)及患者血清中MBL、MASP和C3b的水平,并对这三者之间的水平做相关性分析。结果 A组的MBL水平显著高于C组和D组(P<0.05),G组的MBL水平高于除B组外的其余5组(P<0.05)。F组的MASP水平显著高于A、C、D组,同时其显著低于B、G组(P<0.05),D组的MASP水平显著低于其余6组(P<0.05),G组的MASP水平显著高于其余6组(P<0.05)。D组和F组的C3b水平显著高于A、B、C、E组(P<0.05),但D、F组之间并无显著差异(P>0.05),G组的C3b水平显著低于其余6组(P<0.05),MBL与MASP之间存在中度正相关性,而C3b与MASP、MBL之间存在弱的负相关性(P<0.05)。结论 MBL与机体清除HBV有关,高水平C3b可能会提高乙肝病变程度,MASP水平异常降低与乙肝患者肝损伤程度加重、病毒感染和复制水平加剧均有关系。

七彩神仙鱼C型凝集素家族成员CD302和MBL的克隆及在病原刺激下的免疫应答

七彩神仙鱼(Symphysodon aequifasciatus)具独特的亲代抚育行为,前期研究发现2种C型凝集素在育幼亲本皮肤中高表达,但表达模式不同,预示着潜在的功能分化。为探究两者潜在免疫功能的差异性,克隆获得了七彩神仙鱼C型凝集素基因SaCD302和SaMBL,并分析了病原刺激下的免疫应答模式。结果显示,SaCD302和SaMBL的开放阅读框(ORF)长度分别为741和795 bp,分别编码246和264个氨基酸。SaCD302的氨基酸序列包含一个信号肽(aa 1—29),一个CTL结构域(aa 32—169)和一个跨膜结构域(aa 184—206)。SaMBL的氨基酸序列包含两个低复杂度区域(aa 32—92和aa 104—121)和一个典型的CTL结构域(aa 137—263)。SaCD302和SaMBL的氨基酸序列与尼加拉瓜湖始丽鱼(Archocentrus centrarchus)对应氨基酸序列的同源性最高。SaCD302在各组织中均有表达,头肾中表达量最高,其次为肝脏和鳃;SaMBL在皮肤中高表达,在肠道、肝脏、脾脏和性腺中低表达。嗜水气单胞菌(Aeromonas hydrophila)感染后,SaCD302在脾脏、头肾、肠道和皮肤中的表达量均显著上调,SaMBL仅在头肾、肠道和皮肤中表达上调,且时序性不同,表明二者可能在七彩神仙鱼免疫防御中发挥不同作用。

MBL在甲状腺癌与结节性甲状腺肿的表达及意义

目的:研究甲状腺癌、结节性甲状腺肿患者血清中甘露糖结合凝集素(MBL)的表达水平,探讨其临床意义。方法:选取甲状腺癌患者100例(其中乳头状癌70例,滤泡状癌30例)、结节性甲状腺肿100例,另设健康人120例为对照组,采用ELISA方法分别检测不同组患者及健康人群的外周血血清MBL含量并进行对比分析。结果:甲状腺癌组患者血清MBL表达水平高于结节性甲状腺肿组及对照组,组间比较有统计学差异(P<0.05);结节性甲状腺肿组中血清MBL水平与对照组相比较差异无统计学意义(P>0.05);甲状腺癌合并颈部淋巴结转移与未转移病例的血清MBL水平相比较,差异无统计学意义(P>0.05);甲状腺癌组中,单结节癌灶与结节癌灶患者的血清MBL水平相比较差异无统计学意义(P>0.05)。结论:评估甲状腺结节患者外周血血清MBL的水平,对于区分甲状腺结节良恶性方面有一定的鉴别意义,且患者血清MBL的表达情况与甲状腺癌的病灶数量及是否有淋巴结转移无关。

慢性丙型肝炎患者血浆内毒素和血清MBL变化及临床意义

目的:探讨了慢性丙型肝炎患者血浆内毒素和血清甘露聚糖结合凝集素(MBL)水平的变化及意义。方法:应用鲎试验和酶联法对31例慢性丙型肝炎患者进行了血浆内毒素和血清MBL测定,并与35名正常健康人作比较。结果:慢性丙型肝炎患者血浆内毒素和血清MBL水平均非常显著地高于正常人水平(P<0.01),且内毒素水平与MBL呈正相关(r=0.4784,P<0.01)。结论:血浆内毒素和血清MBL可反映HCV感染导致慢性病理状态,它可能也参与肝脏纤维化的过程。

The binding of MBL to common bacteria in infectious diseases of children

Objective:To purify Mannan-binding lectin(MBL)from human serum and detect its binding ability to several kindsof bacteria common in infections diseases of children.Methods:MBL was purifide from human serum by affinity chromatographyon mannan-Sepharose 4B column.Its binding ability to eight species,97 stratus of bacteria was detected by enzyme-linked lectinassay(ELLA).Results:MBL has different binding ability to bacteria and shows strong binding ability to Klebsiella ornithinolvticaand Escherichia coli,but shows relatively lower binding ability to Staphylococcus haemolyticus,Enterobacter cloacae andStaphylococcus epidermidis.To different isolates of Klebsiella pneumoniae,Haemophilus influenzae and Staphylococcus aureus,MBL shows quite different binding ability.Conclusions:MBL has different binding ability to different bacteria,and has relativelystronger binding ability to Gram-negative bacteria.Its binding ability to different isolates of certain kinds of bacteria is quitedifferent.

The clinical relevance of MBL2 gene polymorphism and sepsis

Objective:To detect the clinical relevance of mannose-binding lectin 2(MBL2) gene polymorphism and sepsis in Chinese lived in Hainan island.Methods: Blood samples from 57 patients with sepsis and 69 patients without sepsis were collected in the ICU of several large hospitals in Hainan province. Genomic DNA was extracted from whole blood and then PCR purification product was sequenced and typed by 3730 sequencing analyzer. The concentration of MBIL2 in serum was detected by ELISA.Results: We found that genotype and allele distributions in two groups were in accordance with the Hardy-Weinberg Equilibrium. The frequency of GA genotype was significantly higher than that in non-sepsis group(P=0.013). A allele frequency in sepsis group was also much higher than that in non-sepsis group(P=0.028).Logister regression analysis showed that the patients who carried A allele were more prone to get sepsis than G allele carrier(P=0.014, OR=2,550, 95%CI=1.207-5.386). The MBL2 level in serum of sepsis patients with genotype GG and GA was significantly lower than that in non-sepsis group(P<0.05). In sepsis group, the MBL2 serum level of patients with genotype GA was obviously lower than that in patients with genotype GG(P<0.05).Conclusions: The variation of rs 1800450 G→A increased the incidence of sepsis and decreased the level of MBL2 in serum.