NLRP3炎性小体研究新进展

NLRP3炎性小体是一种分子量约为700Kda的大分子多蛋白复合体,能被多种病原相关的分子模式或损伤相关的分子模式活化,对固有免疫系统免疫功能的发挥具有极其重要的作用。但如果其被过度激活则可通过活化的半胱天冬酶-1持续地将pro-IL-1β和pro-IL-18剪切为成熟的IL-1β和IL-18,进而激活下游信号转导通路,产生大量的炎性介质,引起机体发生严重的炎症反应,最终促进多种炎症性疾病的发生与发展,如Muckle—wells综合征、2型糖尿病、非酒精性脂肪肝、动脉粥样硬化、炎症性肠病和阿尔兹海默病等。因此,对NLRP3炎性小体进行深入的研究不仅有助于阐释固有免疫系统如何有效地发挥其免疫功能,而且作为系列炎症反应的核心,NLRP3炎性小体：还可能成为多种炎症性疾病防治的新靶点。我们就NLRP3炎性小体的结构与功能,激活与调控,分布与疾病的近期研究作一综：违。     

NLRP3 炎性小体研究新进展

NLRP3 炎性小体是一种分子量约为700Kda 的大分子多蛋白复合体,能被多种病原相关的分子模式或损伤相关的分子模式 活化,对固有免疫系统免疫功能的发挥具有极其重要的作用。但如果其被过度激活则可通过活化的半胱天冬酶-1 持续地将 pro-IL-1茁和pro-IL-18 剪切为成熟的IL-1茁和IL-18,进而激活下游信号转导通路,产生大量的炎性介质,引起机体发生严重的炎 症反应,最终促进多种炎症性疾病的发生与发展,如Muckle-Wells综合征、2 型糖尿病、非酒精性脂肪肝、动脉粥样硬化、炎症性肠 病和阿尔兹海默病等。因此,对NLRP3 炎性小体进行深入的研究不仅有助于阐释固有免疫系统如何有效地发挥其免疫功能,而 且作为系列炎症反应的核心,NLRP3 炎性小体还可能成为多种炎症性疾病防治的新靶点。我们就NLRP3 炎性小体的结构与功 能,激活与调控,分布与疾病的近期研究作一综述。     

NLRP3炎性小体激活调控机制及其在类风湿性关节炎中的潜在作用

NOD样受体热蛋白结构域相关蛋白3(NOD-like receptor family pyrin domain containing 3,NLRP3)炎性小体是一种多蛋白复合物,在非特异性免疫中发挥重要作用,可以通过K+外流、溶酶体损伤、线粒体功能障碍和活性氧生成等途径被激活,产生具有生物活性的白介素-1β(interleukin-1β,IL-1β)、IL-18和肿瘤坏死因子α(tumor necrosis factor alpha,TNF-α),从而导致细胞死亡,激活适应性免疫。NLRP3基因多态性、表达水平、激活状态都与类风湿性关节炎的疾病进程关系密切,并且NLRP3炎性小体异常激活驱动的慢性炎症在类风湿性关节炎发生发展中发挥重要作用。本文就NLRP3炎性小体的分子结构、基本生物学功能及其与类风湿性关节炎疾病进程之间的相关性作一综述,以期为防治该类自身免疫性疾病提供新思路。     

Nek7与NLRP3炎性小体激活机制的研究进展

目前,Nod样受体蛋白3(nod-like receptor protein 3,NLRP3)炎性小体在免疫与人类疾病中的重要性已经得到公认,但NLRP3炎性小体的具体激活机制尚不清楚。NIMA相关蛋白激酶7(NIMA-related kinase 7,Nek7)参与NLRP3炎性小体激活,最终导致白介素IL-1β、IL-18的成熟及分泌。同时Nek7也被证实参与有丝分裂纺锤体形成和中心体的分离,且发现NLRP3炎性小体的激活和有丝分裂不能同时发生。因此,Nek7可能作为有丝分裂和NLRP3炎性小体激活两者之间的转换。本文就Nek7及NLRP3炎性小体的激活关系做一综述,以期为炎症性疾病提供新的治疗方向。     

中药有效成分调控NLRP3 炎症小体活化的研究进展

炎症小体是细胞内组装形成的大分子蛋白复合体,可将白介素-1β(IL-1β) 和IL-18 加工成熟,并诱导细胞焦亡性死亡,在协调对抗病原体感染和生理紊乱的过程中发挥重要作用。Nod 样受体蛋白3(Nod-like receptor protein 3, NLRP3) 炎症小体是迄今为止结构和功能研究得最为明确的炎症小体,其活化后参与免疫性疾病、心血管疾病、神经系统疾病等多种疾病发生及发展过程。研究显示,许多中药有效成分可以调节相关疾病靶细胞中NLRP3 炎症小体的活化。从中药有效成分调节相关疾病靶细胞（如神经细胞、肝肾细胞、内皮细胞、肿瘤细胞等）中NLRP3 炎症小体活化的机制出发,综述近4 年国内外对中药有效成分调节NLRP3 炎症小体活化的研究进展,以期阐释相关中药有效成分的作用特点,并为相关疾病的防治提供一定参考。     

粪肠球菌脂磷壁酸通过 激活NF-κB活化NLRP3炎性体

目的检测粪肠球菌脂磷壁酸(LTA)对NLRP3炎性体的活化机制。方法粪肠球菌LTA及NF-κB抑制剂作用于小鼠巨噬细胞RAW264.7上,运用Western blot及ELISA法检测NLRP3炎性体相关因子mRNA及蛋白的表达,检验LTA对NLRP3的活化是否借助NF-κB信号通路,免疫荧光染色检测NF-κB的核转位。结果LTA可直接活化RAW264.7细胞的NLRP3炎性体。LTA作用于细胞后NLRP3、Caspase-1和IL-1β蛋白的表达明显高于对照组(P0.05)。NF-κB抑制剂可有效抑制NF-κB P65的核转位,而一旦NF-κB信号通路被抑制,NLRP3炎性体蛋白的表达均明显降低。结论 LTA能直接激活小鼠巨噬细胞系RAW264.7的NLRP3炎性体的表达,NF-κB信号通路参与此过程。     

NLRP3炎性小体与脑缺血性损伤

炎性小体是一种蛋白质复合物,作为固有免疫的感受器,在清除病原体感染和有害物质中发挥重要作用。但是,炎性小体的过度活化也是导致自身免疫性疾病和代谢性疾病的主要原因。NLRP3(NLR family,pyrin domain containing 3)炎性小体作为炎性小体中研究最透彻最热门的一种,是炎症反应的核心,在神经系统炎症中发挥了重要作用,并且介导了多种神经变性疾病的发生发展过程。本文综述了NLRP3炎性小体的结构、NLRP3炎性小体在脑缺血性损伤中的作用以及相关调控机制。     

炎性体与器官移植

炎性体是指存在于细胞质内能够激活半胱天冬酶-1（caspase-1）的大分子复合物,活化的caspase-1通过酶切白细胞介素-1β（IL-1β）和白细胞介素-18（IL-18）前体分子而生成具有生物学活性的IL-1β和IL-18.近来研究发现,炎性体分子NLRP1、NLRP2、NLRP5、CARD8、CASP5的基因型与移植的临床结果相关,心脏移植排斥反应时ASC和IL-1β的表达升高,缺血再灌注损伤中NLRP3炎性体激活增加IL-1β分泌,表明炎性体的激活与移植排斥反应和缺血再灌注损伤密切相关,但诱导炎性体活化的配体和参与的炎性体分子有待进一步研究.     

慢性PM2.5暴露对C57BL/6J小鼠肺组织炎症和NLRP3炎性小体活性的影响

目的 研究慢性PM2.5暴露对小鼠肺炎症和NLRP3炎性小体活性的影响,为防治PM2.5所致肺损伤提供新靶点。方法 雄性C57BL/6J小鼠通过不同剂量气管滴注法进行PM2.5染毒,剂量为2,10mg/(kg·bw),对照组小鼠滴注生理盐水。小鼠连续滴注20次,每3d染毒1次后,取血和肺组织。三组小鼠进行血细胞计数;用免疫荧光染色法检测肺组织巨噬细胞水平;用试剂盒测定肺组织中白细胞介素(interleukin,IL)-1β,IL-18水平及caspase-1活性;用实时定量PCR法检测肺组织NLRP3炎性小体相关mRNA表达水平。结果 两个剂量PM2.5染毒均能明显降低单核细胞百分比(P<0.01),增加中性粒白细胞百分比(P<0.01);导致肺炎症发生;增加肺组织caspase-1活性(P<0.01)及NLRP3和ASC的mRNA表达(P<0.01)。与对照组相比,两个剂量组小鼠肺组织IL-1β和IL-18水平均显著增高(P<0.01)。结论 慢性PM2.5暴露可能通过激活肺组织NLRP3炎性小体导致肺炎症发生。     

NLRP3炎症小体在真菌感染中的作用机制研究进展

炎症小体(Inflammasome)是细胞内识别危险信号的多蛋白复合体,是固有免疫的重要组成部分,NOD样受体家族含热蛋白结构域蛋白3炎症小体(NLRP3)是目前研究最多的一种炎症小体。真菌感染中,NLRP3炎症小体通路募集半胱天冬蛋白酶的前体半胱氨酸天冬氨酸蛋白酶1(pro-caspase-1)自身剪切活化,活化后的半胱天冬蛋白酶(Caspase-1),通过对促炎因子IL-1β(interleukin-1β, IL-1β)和IL-18(interleukin-18, IL-18)的激活,引起宿主的炎症反应,在宿主免疫应答中发挥了重要作用。     

Ethylene biosynthesis in Regnellidium diphyllum and Marsilea quadrifolia

The pathway of ethylene biosynthesis was examined in two lower plants, the semi-aquatic ferns Regnellidium diphyllum Lindm. and Marsilea quadrifolia L. As a positive control for the ethylene-biosynthetic pathway of higher plants, leaves of Arabidopsis thaliana (L.) Heynh. were included in each experiment. Ethylene production by Regnellidium and Marsilea was not increased by treatment of leaflets with 1-aminocyclopropane-1-carboxylic acid (ACC), the precursor of ethylene in higher plants. Similarly, ethylene production was not inhibited by application of aminoethoxyvinylglycine and -aminoisobutyric acid, inhibitors of the ethylene biosynthetic enzymes ACC synthase and ACC oxidase, respectively. However, ACC was present in both ferns, as was ACC synthase. Compared to leaves of Arabidopsis, leaflets of Regnellidium and Marsilea incorporated little [¹⁴C]ACC and [¹⁴C]methionine into [¹⁴C]ethylene. From these data, it appears that the formation of ethylene in both ferns occurs mainly, if not only, via an ACC-independent route, even though the capacity to synthesize ACC is present in these lower plants.Abbreviations ACC 1-aminocyclopropane-1-carboxylic acid - AdoMet S-adenosyl-l-methionine - AIB -aminoisobutyric acid - AVG aminoethoxyvinylglycine This research was supported by the U.S. Department of Energy through grant No. DE-FG02-91ER20021 and, in part, by a fellowship of the National Engineering and Research Council of Canada to Jacqueline Chernys.     

Actinotrichia collagens and their role in fin formation

The skeleton of zebrafish fins consists of lepidotrichia and actinotrichia. Actinotrichia are fibrils located at the tip of each lepidotrichia and play a morphogenetic role in fin formation. Actinotrichia are formed by collagens associated with non-collagen components. The non-collagen components of actinotrichia (actinodins) have been shown to play a critical role in fin to limb transition. The present study has focused on the collagens that form actinotrichia and their role in fin formation. We have found actinotrichia are formed by Collagen I plus a novel form of Collagen II, encoded by the col2a1b gene. This second copy of the collagen II gene is only found in fishes and is the only Collagen type II expressed in fins. Both col1a1a and col2a1b were found in actinotrichia forming cells. Significantly, they also expressed the lysyl hydroxylase 1 (lh1) gene, which encodes an enzyme involved in the post-translational processing of collagens. Morpholino knockdown in zebrafish embryos demonstrated that the two collagens and lh1 are essential for actinotrichia and fin fold morphogenesis. The col1a1 dominant mutant chihuahua showed aberrant phenotypes in both actinotrichia and lepidotrichia during fin development and regeneration. These pieces of evidences support that actinotrichia are composed of Collagens I and II, which are post-translationally processed by Lh1, and that the correct expression and assembling of these collagens is essential for fin formation. The unique collagen composition of actinotrichia may play a role in fin skeleton morphogenesis.     

Effect of octanoic acid on ethylene-mediated processes in Arabidopsis

We have examined whether octanoic acid (OA) one of the short chain saturated fatty acids (SCSFA), increases ethylene response in the following three ethylene-mediated processes: a) hypocotyl growth in darkness; b) formation of new flowers; c) flower abscission. These processes were examined in the presence or absence of exogenous ethylene in Arabidopsis wild type (WT) and in the ethylene-insensitive mutants, etr1-3 and ein2-1 and in the ethylene over-producer mutant eto1-1. Our results show that OA decreased hypocotyl length of WT in the absence or presence of exogenous ethylene, apparently showing that OA acts via augmentation of ethylene action. However, the hypocotyl growth inhibition could not be ascribed to increased ethylene sensitivity since application of inhibitors of ethylene synthesis (aminoethoxyvinylglycine; AVG) or action (1-methylcyclopropene;1-MCP) to WT seedlings did not prevent specifically the OA-induced growth inhibition. Also, OA inhibited hypocotyl growth in the mutants etr1-3 and ein2-1 in a similar pattern to that obtained in WT. On the other hand, OA had no effect on flower formation neither in WT, etr1-3 and eto1-1, in which ethylene reduced flower formation, nor in the ein2-1 mutant, in which ethylene had no effect. OA also did not increase flower abscission in WT or in the mutants etr1-3 and ein2-1 neither in the absence nor in the presence of ethylene. However, OA has augmented flower abscission in the mutant eto1-1 only in the absence of exogenous ethylene. This result might indicate that the effect of OA on eto1-1 is specific to this mutant and is not due to general deleterious effects inflicted by OA. Taken together, our results show that in general OA does not augment ethylene response in Arabidopsis, but it might affect ethylene action in flower abscission of the ethylene-overproducer mutant.     

A storage-protein marker associated with the suppressor of Pm8 for powdery mildew resistance in wheat

A suppressor of resistance to powdery mildew conferred by Pm8 showed complete association with the presence of a storage-protein marker resolved by electrophoresis on SDS-PAGE gels. This marker was identified as the product of the gliadin allele Gli-A1a. The mildewresponse phenotypes of wheats possessing the 1BL.1RS translocation were completely predictable from electrophoretograms. The suppressor, designated SuPm8, was located on chromosome 1AS. It was specific in its suppression of Pm8, and did not affect the rye-derived resistance phenotypes of wheat lines with Pm17, also located in 1RS, or of lines with Pm7.     

蛋白-O-岩藻糖基转移酶1基因CfPOFUT1在果生炭疽菌中的功能分析

【目的】蛋白-O-岩藻糖基转移酶1 (protein O-fucosyltransferase 1,POFUT1)是催化蛋白质O-岩藻糖基化的关键酶,在动物和人体内被证明调控一系列的生理病理过程,然而POFUT1基因在果生炭疽菌乃至真菌中还未见报道。本研究旨在克隆果生炭疽菌中CfPOFUT1基因,并分析其生物学功能。【方法】利用RT-PCR技术扩增CfPOFUT1的基因并进行生物信息学分析,构建了CfPOFUT1基因的沉默和过表达载体,通过PEG介导法将载体导入原生质体中获得CfPOFUT1基因的沉默和过表达突变体。测定了野生型菌株、CfPOFUT1沉默菌株和过表达菌株在PDA上的菌丝生长、分生孢子产生、萌发与附着胞形成、胁迫应答和致病力、杀菌剂敏感性等生物学表型。【结果】与野生型菌株相比,基因过表达突变体产孢量显著增加,致病力增强,对嘧菌酯敏感性降低,但对多菌灵和咪鲜胺敏感性增强。基因沉默突变体产孢量减少,细胞壁完整性、内质网应激敏感性提高,致病力减弱,对嘧菌酯敏感性提高,但对多菌灵和咪鲜胺敏感性降低。【结论】CfPOFUT1基因参与调控果生炭疽菌分生孢子产量,细胞壁完整性、内质网对应激和药剂敏感性,并对其致病性也具有一定的影响。     

Ethylene formation from 1-aminocyclopropane-1-carboxylic acid in homogenates of etiolated pea seedlings

Homogenates of etiolated pea (Pisum sativum L.) shoots formed ethylene upon incubation with 1-aminocyclopropane-1-carboxylic acid (ACC). In-vitro ethylene formation was not dependent upon prior treatment of the tissue with indole-3-acetic acid. When homogenates were passed through a Sephadex column, the excluded, high-molecular-weight fraction lost much of its ethylene-synthesizing capacity. This activity was largely restored when a heat-stable, low-molecular-weight factor, which was retarded on the Sephadex column, was added back to the high-molecular-weight fraction. The ethylene-synthesizing system appeared to be associated, at least in part, with the particulate fraction of the pea homogenate. Like ethylene synthesis in vivo, cell-free ethylene formation from ACC was oxygen dependent and inhibited by ethylenediamine tetraacetic acid, n-propyl gallate, cyanide, azide, CoCl₃, and incubation at 40°C. It was also inhibited by catalase. In-vitro ethylene synthesis could only be saturated at very high ACC concentrations, if at all. Ethylene production in pea homogenates, and perhaps also in intact tissue, may be the result of the action of an enzyme that needs a heat-stable cofactor and has a very low affinity for its substrate, ACC, or it may be the result of a chemical reaction between ACC and the product of an enzyme reaction. Homogenates of etiolated pea shoots also formed ethylene with 2-keto-4-mercaptomethyl butyrate (KMB) as substrate. However, the mechanism by which KMB is converted to ethylene appears to be different from that by which ACC is converted.Abbreviations ACC 1-aminocyclopropane-1-carboxylic acid - IAA indole-3-acetic acid - KMB 2-keto-4-mercaptomethyl butyrate - SAM S-adenosylmethionine     

A long region upstream of the IME1 gene regulates meiosis in yeast

Summary Meiosis and sporulation in yeast are subject to two types of regulation. The first depends on environmental conditions. The second depends on a genetic pathway which involves the control of the positive regulatory gene IME1 by RME1, which is in turn controlled by the MAT locus. The presence of IME1 on a multicopy plasmid enables cells to undergo meiosis regardless of their genotype at MAT or RME1. We show here that a multicopy plasmid carrying IME1 also enables meiosis, regardless of the environment. Therefore, both kinds of regulation appear to act through IME1. Furthermore, the behavior of multicopy plasmids carrying various segments from the IME1 region suggests that the region upstream of IME1 contains both positive and negative regulatory sites. Control of IME1 by the environment and by the MAT pathway both act through negative regulatory sites.     

Pigmentation in Black-boned sheep (Ovis aries): association with polymorphism of the MC1R gene

Variations in vertebrate skin and hair color are due to varied amounts of eumelanin (brown/black) and phaeomelanin (red/yellow) produced by the melanocytes. The melanocortin 1 receptor (MC1R) is a regulator of eumelanin and phaeomelanin production in the melanocytes, and MC1R mutations causing coat color changes are known in many vertebrates. We have sequenced the entire coding region of the MC1R gene in Black-boned, Nanping indigenous and Romney Marsh sheep populations and found two silent mutation sites of A12G and G144C, respectively. PCR-RFLP of G144C showed that frequency of allele G in Black-boned, Nanping indigenous and Romney Marsh sheep was 0.818, 0.894 and 0, respectively. Sheep with GG genotype had significantly higher (P < 0.05) tyrosinase activity than sheep with CC genotype in the all investigated samples. Moreover, there was significant effect of MC1R genotype on coat color, suggesting that MC1R gene could affect coat color but not black traits. There would be merit in further studies using molecular techniques to elucidate the cause of black traits in these Black-boned sheep.