Establishment of a Multiplex Detection Method for Common Bacteria in Blood Based on Human Mannan-Binding Lectin Protein-Conjugated Magnetic Bead Enrichment Combined with Recombinase-Aided PCR Technology

Objective Recombinase-aided polymerase chain reaction(RAP)is a sensitive,single-tube,two-stage nucleic acid amplification method.This study aimed to develop an assay that can be used for the early diagnosis of three types of bacteremia caused by Staphylococcus aureus(SA),Pseudomonas aeruginosa(PA),and Acinetobacter baumannii(AB)in the bloodstream based on recombinant human mannanbinding lectin protein(M1 protein)-conjugated magnetic bead(M1 bead)enrichment of pathogens combined with RAP.Methods Recombinant plasmids were used to evaluate the assay sensitivity.Common blood influenza bacteria were used for the specific detection.Simulated and clinical plasma samples were enriched with M1 beads and then subjected to multiple recombinase-aided PCR(M-RAP)and quantitative PCR(qPCR)assays.Kappa analysis was used to evaluate the consistency between the two assays.Results The M-RAP method had sensitivity rates of 1,10,and 1 copies/μL for the detection of SA,PA,and AB plasmids,respectively,without cross-reaction to other bacterial species.The M-RAP assay obtained results for<10 CFU/mL pathogens in the blood within 4 h,with higher sensitivity than qPCR.M-RAP and qPCR for SA,PA,and AB yielded Kappa values of 0.839,0.815,and 0.856,respectively(P<0.05).Conclusion An M-RAP assay for SA,PA,and AB in blood samples utilizing M1 bead enrichment has been developed and can be potentially used for the early detection of bacteremia.

Mannan-binding lectin directly interacts with Toll-like receptor 4 and suppresses lipopolysaccharide-induced inflammatory cytokine secretion from THP-1 cells

Mannan-binding lectin(MBL)plays a key role in the lectin pathway of complement activation and can influence cytokine expression.Toll-like receptor 4(TLR4)is expressed extensively and has been demonstrated to be involved in lipopolysaccharide(LPS)-induced signaling.We first sought to determine whether MBL exposure could modulate LPS-induced inflammatory cytokine secretion and nuclear factor-kB(NF-kB)activity by using the monocytoid cell line THP-1.We then investigated the possible mechanisms underlying any observed regulatory effect.Using ELISA and reverse transcriptase polymerase chain reaction(RT-PCR)analysis,we found that at both the protein andmRNAlevels,treatment withMBLsuppresses LPS-induced tumor-necrosis factor(TNF)-a and IL-12 production in THP-1 cells.An electrophoretic mobility shift assay and western blot analysis revealed that MBL treatment can inhibit LPS-induced NF-kB DNA binding and translocation in THP-1 cells.While the binding of MBL to THP-1 cells was evident at physiological calcium concentrations,this binding occurred optimally in response to supraphysiological calcium concentrations.This binding can be partly inhibited by treatment with either a soluble form of recombinant TLR4 extracellular domain or anti-TLR4 monoclonal antibody(HTA125).Activation of THP-1 cells by LPS treatment resulted in increased MBL binding.We also observed that MBL could directly bind to the extracellular domain of TLR4 in a dose-dependent manner,and this interaction could attenuate the binding of LPS to cell surfaces.Taken together,these data suggest that MBL may affect cytokine expression through modulation of LPS-/TLR-signaling pathways.These findings suggest that MBL may play an important role in both immune regulation and the signaling pathways involved in cytokine networks.

Association of mannan-binding lectin gene polymorphisms with progression of severe lupus nephritis

Objective To investigate the association of single nucleotide polymorphisms(SNPs)of the mannan-binding lectin(MBL)gene with serum levels,development,progression and prognosis of severe lupus nephritis(LN).Methods A total of 107 severe lupus nephritis patients were enrolled in the study from January 2003 to October2013.Integrated capillary electrophoresis was used to detect MBL gene polymorphism in peripheral

胸腔积液沉渣包埋组织TTF-1、Galectin-3的表达水平与肺腺癌恶性生物学行为间的关系

目的探讨胸腔积液沉渣包埋组织甲状腺转录因子1(TTF-1)、半乳糖凝集素-3(Galectin-3)的表达水平与肺腺癌恶性生物学行为间的关系。方法选取2020年10月至2023年3月在该院就诊的肺腺癌患者163例,根据分化程度分为高分化组(26例)、中分化组(78例)、低分化组(59例)。对比3组胸腔积液沉渣包埋组织TTF-1、Galectin-3及恶性生物学行为相关基因(p16基因mRNA)表达水平,Spearman秩相关系数分析胸腔积液沉渣包埋组织TTF-1、Galectin-3与p16基因mRNA表达水平的相关性,多元线性回归分析胸腔积液沉渣包埋组织TTF-1、Galectin-3与p16基因mRNA表达水平间的依存关系,限制性立方样条图分析胸腔积液沉渣包埋组织TTF-1、Galectin-3与p16基因mRNA表达水平间的剂量-效应关系。结果低分化组胸腔积液沉渣包埋组织TTF-1、Galectin-3表达水平高于中分化组、高分化组,p16基因mRNA表达水平低于中分化组、高分化组,中分化组胸腔积液沉渣包埋组织TTF-1、Galectin-3表达水平高于高分化组,p16基因mRNA表达水平低于高分化组,差异有统计学意义(P<0.05);胸腔积液沉渣包埋组织TTF-1(r=-0.752,P<0.001)、Galectin-3(r=-0.811,P<0.001)表达水平与p16基因mRNA表达水平呈负相关;胸腔积液沉渣包埋组织Galectin-3表达水平与p16基因mRNA表达水平间无线性依存关系(P>0.05),胸腔积液沉渣包埋组织TTF-1表达水平与p16基因mRNA表达水平间有线性依存关系(P=0.049);当胸腔积液沉渣包埋组织TTF-1表达水平<4分、胸腔积液沉渣包埋组织Galectin-3表达水平<3分时,对p16基因mRNA表达作用最显著。结论胸腔积液沉渣包埋组织TTF-1、Galectin-3表达水平与肺腺癌恶性生物学行为关系密切,早期检测对临床实现精准干预避免病情恶化具有重要意义。

LPS诱导小鼠脑小胶质细胞的激活及Tomato lectin的表达变化

探讨小胶质细胞对侧脑室注射内毒素脂多糖(lipopolysaccharide,LPS)刺激的反应及时程变化。采用组织化学方法,观察小鼠单次注射LPS入侧脑室后,Tomatolectin阳性的小胶质细胞于不同时间点在脑内的分布及表达的时程变化。LPS注射24h后,Tomatolectin组织化学染色显示血管内皮细胞、静息的和不同激活状态的小胶质细胞均呈阳性反应,其中Tomatolectin阳性的小胶质细胞明显被激活,2d时达表达高峰,巨噬细胞样的细胞和小胶质细胞呈现出肥大的、阿米巴样或杆状细胞等不同激活状态下的形态特征。这些激活的小胶质细胞主要分布于侧脑室周围的脑实质结构,如海马、隔区、胼胝体、纹状体,第三脑室周围的下丘脑及其它间脑结构。本结果提示:LPS能诱导小鼠脑室周围的脑实质内的小胶质细胞被激活,并上调小胶质细胞内Toma-tolectin的表达,这些细胞可能参与脑内刺激的免疫调节。

Cloning and Sequencing of a Lectin Protein Gene from the Roots of Sophora flavescens

A lectin protein(SFL) with molecular weight about 32 kD which markedly agglutinated rabbit and human red blood cells was purified from the roots of Sophora flavescens Ait. This protein, and apparently inhibited the growth of Fusarium vasinfectum Atk., Gibberella saubinetii (Mont.) Sacc., and Piricularia oryzae Cav. A set of degenerate PCR primer was synthesized according to the N-terminal sequence of the purified protein. The full-length cDNA coding the lectin was cloned by RT-PCR and 5'-RACE and sequenced (GenBank AF285121). The deduced amino acid sequence indicates that a preprotein with 284 amino acid residues is firstly translated and then processed to a mature protein with 254 amino acids. A N-Glycosylation site is the Asn 182 residue.

Identification of a Lectin Gene Induced in Rice in Response to Magnaporthe grisea Infection

By mRNA differential display, eight induced cDNAs were obtained from rice leaves infected with an incompatible race 131 of Magnaporthe grisea, and one of these cDNAs was highly similar to salt-induced mannose-binding lectin gene. Using this fragment as a probe, a full length cDNA was isolated from a nice cDNA library, which was constructed using mRNA from the incompatible race-infected leaves. Sequence analysis indicates that the cDNA encodes a protein of 15 kD with 145 amino, acids and shares 96% identity at nucleotide level with MRL and salT, but is identical to MRL at amino acid level. Genomic Southern blotting shows that there are two mannose-binding lectin genes in rice genome. Northern blotting analysis indicates that the gene was strongly and specifically induced in rice leaves infected with the incompatible race, suggesting that the lectin induction be involved in the defense of rice to M. grisea.

Lectin法分析uNK细胞在人妊娠母胎界面的分布变化

通过Lectin法分析uNK细胞在人妊娠早、晚期母胎界面的分布变化。结果发现:(1)在妊娠早期的蜕膜中,uNK细胞主要有两种形式,一种是成熟uNK细胞,细胞体积较大,胞浆和胞膜呈现强烈的棕黄色染色,分布于蜕膜的血管中。另一种是未成熟uNK细胞,细胞体积较小,胞核呈现黄色染色,分布于蜕膜细胞之间。(2)在妊娠早期的绒毛组织中,uNK主要是未成熟uNK,分布于绒毛间质之间。(3)与妊娠早期蜕膜的uNK细胞数相比,至妊娠晚期,蜕膜的uNK细胞数量明显减少(P<0.01)。(4)在妊娠晚期,绒毛组织不表达uNK细胞。结论:uNK细胞主要分布于子宫蜕膜组织,且随着妊娠的进展,其表达数量明显下降。这种时空性的表达变化可能与其在调控滋养层细胞的侵袭、血管重建及免疫耐受方面密切相关。

Transformation of Pea Lectin Gene and Parasponia Haemoglobin Gene into Rice and Their Expressions

Lectin and leghemoglobin in legumes play the important roles, respectively, in recognition of host plants to their rhizobial bacteria, and lowering the oxygen partial pressure around bacteroids and protecting nitrogenase from oxygen in symbiotic nitrogen-fixing nodules. In order to extend the host range of the rhizobial bacteria and to make them fix nitrogen in non-legumes, pea lectin gene (pl) and Parasponia hemoglobin gene ( phl,) have been constructed into a plant expression vector (pCBHUL) and the vector pCBHUL was introduced into rice calli from immature young embryos by particle bombardment. After the calli were regenerated into plantlets on the resistant-selecting media containing hygromycin, they were identified by PCR and Southern blot hybridization. It was indicated that the pi and phb genes were integrated into nucleic genome of the transformed rice plants. GUS activity and the product of the pi gene were determined by GUS staining, Western blot and in situ hybridization at translational level. Eighteen out of 40 plants resistant to hygromycin were positively identified by PCR analysis with the rate of 45%. The pi gene was expressed in 3 out of 18 plants with 17% and 7.5% in 40 plants. The results may provide a clue for exploring whether Rhizobium leguminosarum by. viceae could extend its host range and make the transgenic rice plants have the possibility of being symbiotic, or associative to nitrogen fixation.

Research on the Lectin in Muscle Tissue of Varicorhinus macrolepis

[Objective] The paper aimed at researching lectins in muscles of Varicorhinus macrolepis and providing scientific basis for researching the adaptation mechanism and immune response of V.macrolepis to environment,which were advantageous for the protection and reproduction of V.macrolepis.[Method] V.macrolepis was used as test materials for the hemagglutination test by dialdehyde fixation to prove the existence of lectins in muscle crude homogenate of Varicorhinus macrolepis and study the physical and chemical characters.[Result] Lectins in muscle crude homogenate of V.macrolepis had shown hemagglutination effects on erythrocytes of six types of animals and had the maximum hemagglutination activity against rabbit erythrocytes,which belonged to the S-type lectins with optimal pH ranged from 4 to 8 and optimal temperature at 60 ℃.Results from the saccharide inhibition test had indicated that the sucrose was the only kind of saccharide which had inhibited the hemagglutination,suggesting that sucrose had played an important role in the process of recognition and aggregation of lectins.[Conclusion] It had been speculated that the optimal pH ranges for thermal sensitivity and hemagglutination activity of lectins in different types of aquatic organisms were similar.

斑节对虾1种lectin基因的电子克隆及分析

以中国明对虾的c-lectin(DQ167572)基因为探针,搜索EST数据库,获得了日本对虾的1个lectin序列,通过电子克隆扩增到了该基因,并对基因进行了生物信息学分析。

蒙药嘎日迪-13对脑缺血大鼠不同时相海马中IL-1β IL-8、ICAM-1、P-selectin表达的影响

目的观察蒙药嘎日迪-13对脑缺血大鼠不同时相海马中IL-1β、IL-8、ICAM-1、P-selectin表达的影响。方法 360只雄性SD大鼠随机分为脑缺血模型组、假手术组、嘎日迪-13大、中、小剂量组,每组又随机分为6个时相组,灌胃给药,一次/d,连续27 d后,线栓法制备大鼠大脑中动脉栓塞模型,神经功能评分后免疫组化法测定海马IL-1β、IL-8、ICAM-1、P-selectin的表达。结果嘎日迪-13明显降低脑缺血大鼠神经功能评分,并明显降低脑缺血大鼠海马IL-1β、IL-8、ICAM-1、P-selectin的表达水平。结论蒙药嘎日迪-13对大鼠脑缺血有较好的保护作用,其机制可能与降低IL-1β、IL-8、ICAM-1、P-selectin等因子的表达水平有关。

豌豆早期结瘤素基因ENOD12A的克隆及与PsLectin基因双元表达载体的构建

采用PrimStar HS DNA聚合酶从豌豆基因组DNA中扩增出了豌豆早期结瘤素基因PsENOD12A.序列分析结果表明,所克隆的基因与GenBank公布的序列仅相差1个碱基,但推导的氨基酸序列没有改变.将PsENOD12A基因和豌豆凝集素基因psl重组进了双元表达载体.

中国明对虾C-型凝集素基因(Fclectin)的重组表达及活性分析

研究拟通过分析对虾C型凝集素的活性特点,探讨其在对虾先天免疫应答过程中的潜在功能以及在养殖生产实践中的应用。实验利用原核表达系统对中国明对虾C-型凝集素基因的两个串联的糖识别结构域(carbohydrate recognition domain,CRD)进行了重组表达,并通过纯化复性获得了重组目的蛋白(rFclectin-CRD1和rFclectin-CRD2)。活性分析结果显示,重组目的蛋白对多种病原菌有凝集和抑制生长的作用,并且具有Ca2+依赖活性;其凝集活性可被半乳糖、肽聚糖、脂多糖等多种病原相关分子模式所抑制,研究结果证实,Fclectin是一种典型的C-型凝集素,它可能作为中国明对虾先天免疫中重要的模式识别受体,在一定程度上参与了机体应答病原微生物的防御过程。

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。

巨蛎属(Crassostrea)四种牡蛎精子Bindin蛋白海藻糖凝集素结构域(Fucose binding lectin)多样性研究

提取巨蛎属中熊本牡蛎、葡萄牙牡蛎和日本巨牡蛎的基因组DNA,应用PCR技术扩增了三种牡蛎的海藻糖凝集素结构域(Fucose binding lectin,F-lectin),结合GenBank中长牡蛎海藻糖凝集素结构域的序列利用邻接法对得到的序列进行了系统进化分析,并利用非同义替换率和同义替换率之间的比值分析了巨蛎属四种牡蛎海藻糖凝集素结构域上可能的受正选择的位点。结果表明,四种巨蛎属牡蛎的海藻糖凝集素结构域序列中长牡蛎与葡萄牙牡蛎的F-lectin比长牡蛎与熊本牡蛎的关系更近,葡萄牙牡蛎三种单倍型(an1,an2,an3)定位在不同的支上,an1与长牡蛎海藻糖凝集素结构域的关系更近,an2与an3与熊本牡蛎之间的关系更近。在巨蛎属中,海藻糖凝集素结构域的3D模型中,发现五个可能的受正向选择的位点(40,66,67,123,125),并且这五个位点都围绕在三个重要的识别氨基酸(H37,R64,R70)周围,推测这五个正向选择位点也许与牡蛎种特异的受精识别有关。

人P-选择素胞外区Lectin片段真核表达载体的构建与鉴定

目的 构建人P 选择素 (P selectin)胞外区凝集素 (Lectin)片段的真核表达载体。方法 从人血小板中提取总RNA ,经RT PCR得到P 选择素cDNA基因 ,用PCR方法扩增其中的Lectin片段 ,并将其克隆到真核表达载体 pcDNA4/HisMaxA中 ,构建了PCMV 启动控制基因表达质粒 pcDNA4/HisMaxA P selectin’sLectin。结果 通过酶切和基因序列分析确定重组入载体 pcDNA4/HisMaxA的片段为目的基因的核苷酸序列。 结论 重组质粒 pcDNA4/HisMaxA P selectin’sLectin的成功构建 ,为在真核细胞中高效表达该表位片段对应蛋白并制备其抗体作进一步研究提供基础。

呼吸系统功能状态与sICAM-1、sVCAM-1、E-selectin的相关性

目的探讨呼吸系统功能状态与E-选择素(E-selectin)、可溶性细胞间黏附分子1(soluble inte FAellular adhesion molecule-1,sICAM-1)、可溶性血管细胞黏附分子1(souble vascular cell adhesion molecule 1,sVCAM-1)的相关性。方法选取体检中心健康体检者216名,根据HRA系统检测的呼吸系统功能状态的结果,将研究对象分为呼吸功能正常组,呼吸功能轻度改变组,支气管、呼吸道炎性反应状态组三组,分别编号为A、B、C组。清晨空腹采血,留取血清,测定sICAM-1、sVCAM-1、Eselectin的含量。结果与A组相比,吸烟使B、C组呼吸系统功能状态改变的危险性增大(OR=1.216,95%CI:0.6~2.466;OR=3.2,95%CI:1.502~6.819)。随着呼吸系统功能状态炎性程度的增加,E-selectin、sICAM-1、sVCAM-1的浓度明显增高,且差异有统计学意义(P均<0.01)。A组中E-selectin、sICAM-1、sVCAM-1的浓度在吸烟组和非吸烟组的差异均无统计学意义;B组中,与非吸烟组相比,吸烟组sICAM-1、sVCAM-1明显增高(P均<0.01);在C组中,吸烟组中E-selectin、sICAM-1、sVCAM-1明显高于非吸烟组,且差异均有统计学意义(P均<0.01)。结论随着呼吸系统功能状态严重程度的增高,E-selectin、sICAM-1、sVCAM-1的浓度明显增高。吸烟者血清E-selectin、sICAM-1、sVCAM-1的水平增加。

Probing Lectin Receptors on the Plasma Membrane of Isolated Viable Generative Cells in Angiosperms by Means of Single Cell Manipulation

Fluorescein isothiocyanate (FITC) conjugated concanavalin agglutinin (Con A), wheat germ agglutinin (WGA) and soybean agglutinin (SBA) were used as probes to localize their specific receptors on the plasma membrane of generative cells (GCs) isolated from Vicia faba L., Iris tectorium Maxim. and Hippeastrum vittatum Herb. It is a further investigation on possible distributive dynamic of lectin receptors during the developmental process from generative cells to sperm cells. In the present study, all the three lectin receptors were found on the surface of generative cells of V faba and I. tectorium. However, on generative cells of H vittatum only Con A and WGA, but not SBA receptors were observed. The same lectin receptors on the generative cells from different species showed various distribution patterns. The distribution of various lectin receptors on the same generative cells also showed different characteristics. Lectin receptors were totally absent on some generative cells of all three investigated species. Polar distribution of lectin receptors was observed on tailed generative cells. The findings offer important clues to investigate sperm cell function and possible sperm dimorphism of surface glycoprotein.

Researches on Extraction,Purification Technique and Properties of Lectin from Porphyra yezoensis

[Objective] The aim was to explore the extraction technique and purification method of lectin from Porpya yezoensis,as well as to investigate the properties of lectin. [Method] The effects of four factors such as buffer system,solid-liquid ratio,temperature,and extracting time on the lectin extraction result from P. yezoensis were investigated by the use of specific activity as the indicator. Then the lectin was purified by DEAE-Sepharose FF chromatography. The hemagglutination activity was used as the indicator,and the properties of the lectin such as carbohydrate specificity,divalent cations dependence,temperature,acidic and alkaline stability and others were detected. [Result] The optimal extraction conditions were：extraction ageat Tris-HCl buffer （25 mmol/L,pH=7.5 ）,solid-liquid ratio of 1：5,extracting temperature of 40 ℃,and extracting time of 16 h. The activity of the lectin of P. yezoensis didn＇t change after 30 min of being heated at 50 ℃,which showed a certain extent of thermal stability,and the suitable pH value was 7-9. The lectin of P. yezoensis could combine with maltose,D-galactose,D-xylose and L-Arabinose,in which the binding force with the maltose was the strongest. The lectin activity was depended on the addition of Ca2＋ and Mg2＋. [Conclusion] The research had provided theoretical basis for the clarification of immune mechanism of P. yezoensis,as well as its high effective utilization.