赤点石斑鱼LECT2基因的克隆与组织表达分析

基于LECT2的EST序列设计特异引物,采用RACE技术,成功克隆获得赤点石斑鱼LECT2 cDNA全序列,全长601 bp,包括了79 bp的3′UTR区、468 bp的开放阅读框（ORF）以及54 bp的5′UTR区,共编码155个氨基酸.通过与21个物种的氨基酸序列进行同源比对发现,所推导氨基酸序列与大黄鱼的相似性最高,为78%,与其他物种的相似性在40%~73%之间,表明LECT2氨基酸序列具有较高的保守性.基于LECT2基因的氨基酸序列构建的脊椎动物系统进化树与传统物种树基本吻合.同时,通过RT-PCR方法得出,LECT2在健康赤点石斑鱼多种组织中均有表达,肝组织表达量最高,感染哈维氏弧菌（Vibrio barveyi）后LECT2在脾、头肾、鳃等免疫器官中有较高表达量,而在肝脏中表达量上调最为显著,其结果证实了LECT2与赤点石斑鱼免疫应答相关,肝脏可能是赤点石斑鱼LCET2蛋白最主要的表达场所.

PaCLR介导PaLECT2激活脂多糖刺激的香鱼(Plecoglossus altivelis)单核巨噬细胞功能

香鱼(Plecoglossus altivelis)白细胞衍生趋化因子2(leukocyte cell-derived chemotaxin 2,PaLECT2)可以激活香鱼头肾来源的单核巨噬细胞(monocytes/macrophages,MO/MΦ),提高细菌感染后香鱼存活率。进一步研究显示,PaLECT2与香鱼C型凝集素受体(C-type lectin receptor,PaCLR)相互作用可激活静息状态下香鱼MO/MΦ,增强其免疫活性。在前期基础上,本研究通过抗体封闭实验检测PaCLR是否介导PaLECT2激活LPS刺激的MO/MΦ功能。结果显示,重组PaLECT2成熟肽(rPaLECT2m)显著提高了LPS刺激的香鱼MO/MΦ细胞因子的表达,并增强了其吞噬能力和杀菌活性。封闭PaCLR显著抑制了rPaLECT2m激活LPS刺激的香鱼MO/MΦ细胞因子表达、吞噬和杀菌功能。因此,PaCLR介导PaLECT2可以激活病理状态香鱼MO/MΦ。这一认识进一步揭示了LECT2在病理状态的鱼类巨噬细胞调控和炎症反应中的作用及机制。

虹鳟LECT2的酵母表达、纯化及生物活性分析

白细胞衍生趋化因子2(leukocyte cell-derived chemotaxin2,LECT2)是一个参与多种生理和病理过程的分泌型细胞因子。该文采用毕赤酵母表达体系分泌表达虹鳟LECT2,用阳离子交换柱结合分子筛层析方法分离纯化目的蛋白,并获得纯度为96%,得率为120mg/L的重组虹鳟(Oncorhynchus mykiss)LECT2酵母培养物。生物学活性验证表明该重组蛋白能趋化虹鳟头肾来源的巨噬细胞,增强其呼吸爆发和杀菌能力,并改变其细胞因子等基因的表达。综上,该实验建立了一种快速有效的虹鳟LECT2活性重组蛋白的制备方法,为后续相关蛋白的功能研究奠定了基础。

香鱼LECT2基因的克隆及其组织表达差异

LECT2(leukocyte cell-derived chemotaxin 2)是一个多功能的蛋白质,其与细胞生长、分化、损伤修复及免疫等过程相关。本研究通过设计简并引物,从香鱼肝脏cDNA文库中筛选LECT2基因,该基因cDNA序列全长547个核苷酸,3'末端具有polyA尾,单一大开读框编码一个由156个氨基酸组成的分子量为17kDa的蛋白质。序列分析及系统进化树分析均表明,香鱼LECT2与虹鳟LECT2最相似,且各物种LECT2的进化关系与目前接受的物种分类关系基本一致。香鱼LECT2基因在香鱼许多组织中均有表达,而肝脏中的表达量最高,肾脏和脑中的表达量也较高。

双荧光素酶报告基因检测斑马鱼c-Myb与lect2l的靶标关系

目的:构建斑马鱼lect2l基因启动子双荧光报告基因系统,研究lect2l是否是受c-Myb蛋白特异性调控的靶基因。方法:采用PCR方法克隆斑马鱼lect2l基因启动子序列,构建重组荧光素酶报告基因载体pGL4.20-lect2lp,并采用阳离子脂质体法将其与c-myb表达载体及pRL-CMV内参质粒共转染293T细胞,使用化学发光仪检测荧光强度并计算比值。结果:电泳显示酶切条带符合斑马鱼lect2l基因启动子序列长度,构建的重组荧光素酶报告基因质粒pGL4.20-lect2lp荧光素酶活性的表达是对照组的30.34倍。结论:斑马鱼lect2l基因启动子驱动的荧光素酶表达载体pGL4.20-lect2lp构建成功,双荧光素酶报告基因系统提示斑马鱼c-Myb蛋白对lect2l基因有转录激活作用。

(TGF)-β1、LECT2在胆道闭锁肝纤维化中的表达水平及诊断价值

目的探究转化生长因子β1(TGF-β1)、白细胞衍生趋化因子2(LECT2)在胆道闭锁肝(BA)纤维化中的表达水平及诊断价值。方法收集2019年2月-2020年8月期间我院收治的50例胆道闭锁患儿及30例胆管扩张症患儿的临床资料,另外选择无肝胆疾病的肝脏组织的28例患儿作为对照组,分别作为胆道闭锁组(n=50)、胆管扩张组(n=30)、对照组(n=28),术中取各组患儿肝右叶前缘为活检标本,HE及免疫组化染色显微镜下观察肝组织细胞发育、肝纤维化程度,进行定性分析、定量分析,取相同倍数显微镜下图片,图像分析软件IPP6.0分析每张图片5个视野,计算TGF-β1、LECT2的AOD。结果胆道闭锁组TGF-β1、LECT2阳性率较胆管扩张组及对照组高(P<0.05),TGF-β1、LECT2表达水平较胆管扩张组及对照组高(P<0.05),Ⅰ级~Ⅱ级患者TGF-β1表达水平明显升高,Ⅲ级~Ⅳ级者TGF-β1表达水平明显降低(P<0.05)。I级~IV级患者随着纤维化程度升高,LECT2表达水平逐渐升高(P<0.05)。病情轻重概率模型为Logit(P)=(-2.954)+1.644BNP+1.843TGF-β1。结论在纤维化早期TGF-β1表达水平明显升高,在晚期TGF-β1表达水平明显下降,LECT2表达水平与肝纤维化程度间具有正向相关性,两者是评估BA患者肝纤维化程度的有效指标。

乌鳢白细胞衍生趋化因子LECT2互作蛋白的筛选与鉴定

为了解乌鳢(Channa argus)白细胞衍生趋化因子2(CaLECT2)在抗菌免疫过程中所调控的配体蛋白,克隆获得CaLECT2基因,并对其表达特征进行了分析。利用体内注射试验分析了CaLECT2对乌鳢机体的免疫增强作用。利用His-pull down联合质谱、Co-IP分析了CaLECT2的互作蛋白。结果显示,在感染鰤诺卡氏菌的乌鳢脾脏、肾脏和肝脏中,CaLECT2 mRNA的表达量显著上调。利用原核表达系统表达纯化获得了CaLECT2重组蛋白。通过Western Blot证明rCaLECT2抗血清可以特异性识别CaLECT2重组蛋白。向乌鳢体内注射CaLECT2蛋白可以显著提高脾脏内巨噬细胞数量。Pull down联合质谱鉴定得到Fetuin-like protein、Serotransferrin和CD209等253个潜在的互作蛋白。Co-IP结果进一步确认了CaLECT2与CD209存在互作关系。研究为深入探讨CaLECT2所调控的配体蛋白功能奠定了前期基础。

Localized production of LECT2 by orthotopic histiocytes during inflammation

Leukocyte cell-derived chemotaxin 2(LECT2),initially identified as a multifunctional protein secreted by hepatocytes and involved in diverse hepatic pathophysiological processes(Yamagoe et al.,1998;Xie et al.,2022),is also a prominent amyloid fibril protein in both renal and hepatic amyloidosis(Mann et al.,2022).Recently,LECT2 has been implicated in immune processes across various pathologies,including hepatocellular carcinoma(HCC),nonalcoholic fatty liver disease(NAFLD),sepsis,atherosclerosis,arthritis,and allergic diseases(Zhu et al.,2023).

Leukocyte cell-derived chemotaxin 2(LECT2)regulates liver ischemia-reperfusion injury

Background and aim Hepatic ischemia–reperfusion injury(IRI)is a significant challenge in liver transplantation,trauma,hypovolemic shock,and hepatectomy,with limited effective interventions available.This study aimed to investigate the role of leukocyte cell-derived chemotaxin 2(LECT2)in hepatic IRI and assess the therapeutic potential of Lect2-short hairpin RNA(shRNA)delivered through adeno-associated virus(AAV)vectors.Materials and methods This study analyzed human liver and serum samples from five patients undergoing the Pringle maneuver.Lect2-knockout and C57BL/6J mice were used.Hepatic IRI was induced by clamping the hepatic pedicle.Treatments included recombinant human LECT2(rLECT2)and AAV-Lect2-shRNA.LECT2 expression levels and serum biomarkers including alanine aminotransferase(ALT),aspartate aminotransferase(AST),creatinine,and blood urea nitrogen(BUN)were measured.Histological analysis of liver necrosis and quantitative reverse-transcription polymerase chain reaction were performed.Results Serum and liver LECT2 levels were elevated during hepatic IRI.Serum LECT2 protein and mRNA levels increased post reperfusion.Lect2-knockout mice had reduced weight loss;hepatic necrosis;and serum ALT,AST,creatinine,and BUN levels.rLECT2 treatment exacerbated weight loss,hepatic necrosis,and serum biomarkers(ALT,AST,creatinine,and BUN).AAV-Lect2-shRNA treatment significantly reduced weight loss,hepatic necrosis,and serum biomarkers(ALT,AST,creatinine,and BUN),indicating therapeutic potential.Conclusions Elevated LECT2 levels during hepatic IRI increased liver damage.Genetic knockout or shRNA-mediated knockdown of Lect2 reduced liver damage,indicating its therapeutic potential.AAV-mediated Lect2-shRNA delivery mitigated hepatic IRI,offering a potential new treatment strategy to enhance clinical outcomes for patients undergoing liver-related surgeries or trauma.

Leukocyte cell-derived chemotaxin 2 inhibits development of atherosclerosis in mice

Leukocyte cell-derived chemotaxin 2 (LECT2), a multifunctional hepatokine, is involved in many pathological conditi ons. However, its role in atherosclerosis remains undefined. In this study, we admimistered vehicle or LECT2 to male Apoe^-/- mice fed a Western diet for 15 weeks. Atherosclerotic lesions were visualized and quantified with Oil-red O and hematoxylin staining. The mRNA expression levels of MCP-1, MMP-1, IL-8 IL-1β, and TNF-a were analyzed by quantitative real-time polymerase chain reaction. Serum TNF-a, IL-1β, IL-8, MCP-1, and MMP-1 concentrations were measured by en zyme-li nked immuno sorbent assay. CD68, CD31, and a-SMA, markers of macrophages, endothelial cells, and smooth muscle cells, respectively, were detected by immuno staining. Results showed that LECT2 reduced total cholesterol and low-density lipoprotein concentrations in serum and inhibited the development of atherosclerotic lesions, accompanied by reductions in inflammatory cytokines and lower MCP-1, MMP-1, TNF-a, IL-8, and IL-1β mRNA abundanee. Furthermore, LECT2 decreased CD68, but in creased cr SMA in atherosclerotic lesi ons, suggesting an in crease in smooth muscle cells and reduction in macrophages. In summary, LECT2 inhibited the development of atherosclerosis in mice, accompanied by reduced serum total cholesterol concentration and lower inflammatory responses.

白细胞衍生趋化因子2及其受体介导的信号通路与疾病

白细胞衍生趋化因子2(leukocyte cell-derived chemotaxin-2,LECT2)属于肽酶M23家族,是具有趋化作用的蛋白质。LECT2能趋化免疫细胞吞噬病原微生物,抑制癌细胞的迁移,对多种疾病如肝癌、败血症、动脉粥样硬化均有重要作用。为了深入了解LECT2在疾病中的作用机制,本文对LECT2基因和蛋白质的结构、与间质表皮转化因子(mesenchymal epithelial transition factor,MET)、C型凝集素等受体的识别机制,在β-联蛋白、Wnt等信号通路中的调节作用,以及与多种疾病的关系进行综述。

孤儿受体调控慢性肝病的研究进展

脂肪堆积过多、生物钟失调、病毒感染、持续炎症反应等可造成肝脏炎症、纤维化、癌变,促进慢性肝病的发展。深入了解导致慢性肝病的病因,以及影响其发生和发展的基本机制,有助于确定潜在的治疗目标,进行靶向治疗。孤儿受体(orphan nuclear receptors, ONRs)是指无相应内源性配体与其结合的受体,对ONRs及其生物学特性的研究促进了合成配体的发展,对研究治疗多种疾病的有效靶点具有重要作用。近年来,研究发现ONRs对于维持正常的肝脏功能至关重要,其功能障碍可影响各种肝脏疾病。ONRs可通过调控激素、转录因子,影响生物钟、氧化应激等方式,影响肝脏脂质代谢、炎症反应、癌细胞增殖等病理生理学活动。基于此,本文重点介绍维甲酸相关孤儿受体(retinoid related orphan nuclear receptors,RORs)亚家族、孕烷X受体(pregnaneXreceptor,PXR)、白细胞衍生的趋化因子2(leukocytecellderivedchemotaxin2,LECT2)、核受体Nur77、肝细胞核因子4α (hepatocyte nuclear factor 4α, HNF4α)这些ONRs通过不同的方式调控不同类型慢性肝病的发生和发展,为基于ONRs调控慢性肝病治疗策略提供有益参考。