Thioredoxin and glutaredoxin-mediated redox regulation of ribonucleotide reductase

Ribonucleotide reductase(RNR), the rate-limitingenzyme in DNA synthesis, catalyzes reduction of thedifferent ribonucleotides to their corresponding deoxyri-bonucleotides. The crucial role of RNR in DNA synthesishas made it an important target for the development ofantiviral and anticancer drugs. Taking account of the re-cent developments in this field of research, this reviewfocuses on the role of thioredoxin and glutaredoxin sys-tems in the redox reactions of the RNR catalysis.

Selenium and the Thioredoxin and Glutaredoxin Systems

Thioredoxin (Trx) is a small ubiquitous dithiol protein which together with the FADcontaining enzyme thioredoxin reductase (TR) and NADPH (the Trx system) is a hydrogen donor for ribonucleotide reductase essential for DNA synthesis and a general protein disulfide reductase involved in redox regulation. Selenite, selenodiglutathione (GS-Se-SG) and selenocystine are efficiently reduced by thioredoxins and also directly by NADPH and mammalian TR but not by the E. coli enzyme. Incubation of selenite or GS-Se-SG with the Trx system or with mammalian TR results in a rapid formation of selenide, which by redox cycling with oxygen may cause a large non-stoichiometric oxidation of NADPH. Selenocystine is efficiently reduced into two molecules of the selenol amino acid selenocysteine by mammalian TR with a Km-value (6μmol·L-1 ) and a high turnover number (kcat, 3200 min-1) almost identical to the natural substrate Trx-S2. TR also directly reduces lipid hydroperoxides and this peroxidase reaction is strongly stimulated by the presence of catalytic amounts of free selenocysteine. Glutaredoxin (Grx) which catalyzes GSH dependent disulfide reduction also via a redox-active disulfide and Trx are both efficient electron donors to the hut-nan plasrna glutathione peroxidase providing a mechanism by which human plasma glutathione peroxidase may reduce hydroperoxides in an environment almost free from glutathione. Selenate is reduced by Grx and Trx in the presence of GSH. The DNA-binding of the transcription factor AP-1 is strongly inhibited by GS-Se-SG and selenite. Furtherrnore, selenide formed by TR-mediated reduction of selenite and GS-Se-SG inhibits lipoxygenase and changes the electron spin resonance spectrum of the active site iron. Mammalian TR with two subunits of 57 kDa has recently been cloned and shown to be homologous to glutathione reductase. The rat enzyme contains a selenocysteine residue in a unique Cterminal position and a conserved SEClS sequence directing insertion of the selenocysteine. The discovery of selenocysteine in mammalian TR may explain the broad substrate specificity of the enzyme and the requirement of seleflium for cell proliferation

Conserved Functions of Arabidopsis and Rice CC-Type Glutaredoxins in Flower Development and Pathogen Response

Glutaredoxins （GRXs） are ubiquitous oxidoreductases that play a crucial role in response to oxidative stress by reducing disulfides in various organisms. In planta, three different GRX classes have been identified according to their active site motifs. CPYC and CGFS classes are found in all organisms, whereas the CC-type class is specific for higher land plants. Recently, two Arabidopsis CC-type GRXs, ROXY1 and ROXY2, were shown to exert crucial functions in petal and anther initiation and differentiation. To analyze the function of CC-type GRXs in the distantly related monocots, we isolated and characterized OsROXY1 and OsROXY2-two rice homologs of ROXY1. Both genes are expressed in vegetative and reproductive stages. Although rice flower morphology is distinct from eudicots, OsROXY1/2 floral expression patterns are similar to their Arabidopsis counterparts ROXY1/2. Complementation experiments demonstrate that OsROXY1 and OsROXY2 can fully rescue the roxyl floral mutant phenotype. Overexpression of OsROXY1, OsROXY2, and ROXY1 in Arabidopsis causes similar vegetative and reproductive plant developmental defects. ROXY1 and its rice homologs thus exert a conserved function during eudicot and monocot flower development. Strikingly, overexpression of these CC-type GRXs also leads to an increased accumulation of hydrogen peroxide levels and hyper-susceptibility to infection from the necrotrophic pathogen Botrytis cinerea, revealing the importance of balanced redox processes in flower organ develop- ment and pathogen defence.

Repression of the Arabidopsis thaliana Jasmonic Acid/Ethylene-Induced Defense Pathway by TGA-Interacting Glutaredoxins Depends on Their C-Terminal ALWL Motif

Glutaredoxins are small heat-stable oxidoreductases that transfer electrons from glutathione （GSH） to oxi- dized cysteine residues, thereby contributing to protein integrity and regulation. In Arabidopsis thaliana, floral glutare- doxins ROXY1 and ROXY2 and pathogen-induced ROXY19/GRX480 interact with bZIP transcription factors of the TGACG （TGA） motif-binding family. ROXY1, ROXY2, and TGA factors PERIANTHIA, TGA9, and TGA10 play essential roles in floral development. In contrast, ectopically expressed ROXY19/GRX480 negatively regulates expression of jasmonic acid （JA）/ ethylene （ET）-induced defense genes through an unknown mechanism that requires clade II transcription factors TGA2, TGA5, and/or TGA6. Here, we report that at least 17 of the 21 land plant-specific glutaredoxins encoded in the Arabidopsis genome interact with TGA2 in a yeast-two-hybrid system. To investigate their capacity to interfere with the expression of JA/ET-induced genes, we developed a transient expression system. Activation of the ORA59 （OCTADECANOID-RESPONSIVE ARABIDOPSIS AP2/ERF-domain protein 59） promoter by transcription factor EIN3 （ETHYLENE INSENSITVE 3） was sup- pressed by co-expressed ROXY19/GRX480. Suppression depended on the L＊＊LL motif in the C-terminus of ROXY19/ GRX480. This putative protein interaction domain was recently described as being essential for the TGA/ROXY interaction. Ten of the 17 tested ROXY proteins suppressed ORA59 promoter activity, which correlated with the presence of the C-terminal ALWL motif, which is essential for ROXY1 function in flower development. ROXY19/GRX480-mediated repres- sion depended on the GSH binding site, suggesting that redox modification of either TGA factors or as yet unknown target proteins is important for the suppression of ORA59 promoter activity.

Monothiol Glutaredoxin-BolA Interactions： Redox Control of Arabidopsis thaliana BolA2 and SufE1

A functional relationship between monothiol glutaredoxins and BolAs has been unraveled by genomic analyses and in several high-throughput studies. Phylogenetic analyses coupled to transient expression of green fluo- rescent protein （GFP） fusions indicated that, in addition to the sulfurtransferase SufE1, which contains a C-terminal BolA domain, three BolA isoforms exist in Arabidopsis thaliana, BolA1 being plastidial, BolA2 nucleo-cytoplasmic, and BolA4 dual-targeted to mitochondria and plastids. Binary yeast two-hybrid experiments demonstrated that all BolAs and SufE 1, via its BolA domain, can interact with all monothiol glutaredoxins. Most interactions between protein couples of the same subcellular compartment have been confirmed by bimolecular fluorescence complementation. In vitro experiments indicated that monothiol glutaredoxins could regulate the redox state of BolA2 and SufE1, both proteins possessing a single conserved reactive cysteine. Indeed, a glutathionylated form of SufE1 lost its capacity to activate the cysteine desuifurase, Nfs2, but it is reactivated by plastidial glutaredoxins. Besides, a monomeric glutathionyiated form and a dimeric disulfide-bridged form of BolA2 can be preferentially reduced by the nucleo-cytoplasmic GrxS17. These results indicate that the glutaredoxin-BolA interaction occurs in several subcellular compartments and suggest that a redox regulation mechanism, disconnected from their capacity to form iron-sulfur cluster-bridged heterodimers, may be physiologically relevant for BolA2 and SufE1.

Glutathione regulates the transfer of iron-sulfur cluster from monothiol and dithiol glutaredoxins to apo ferredoxin

Holo glutaredoxin(Grx)is a homo-dimer that bridges a[2Fe-2S]cluster with two glutathione(GSH)ligands.In this study,both monothiol and dithiol holo Grxs are found capable of transferring their iron-sulfur(FeS)cluster to an apo ferredoxin(Fdx)through direct interaction,regardless of FeS cluster stability in holo Grxs.The ligand GSH molecules in holo Grxs are unstable and can be exchanged with free GSH,which inhibits the FeS cluster transfer from holo Grxs to apo Fdx.This phenomenon suggests a novel role of GSH in FeS cluster trafficking.

Molecular characterization of glutaredoxin 2 from Ostrinia furnacalis

Glutaredoxins(GRXs)play very important roles in maintaining intracellular redox homeostasis.In the present study,the full-length cDNA sequence encoding GRX2,named OfurGRX2(GenBank accession no.GU393246),was obtained from Ostrinia furnacalis,using reverse transcription polymerase chain reaction and rapid amplification of cDNA ends.Sequence analysis revealed that the open reading frame of OfurGRX2 consists of 351 nucleotides encoding 116 amino acid residues with a predicted molecular weight of 12.6 kDa.Homolog research revealed that OfurGRX2 shares a common active site,CPYC/CPFC,with other insect counterparts.Expression profiles revealed that OfurGRX2 is a ubiquitous gene expressed in insect heads,fat bodies,epidermises,mid guts and muscles.The OfurGRX2 transcript peaked in 36-h larvae of 4th instars,and then suddenly declined in the molting stage.Hormone treatment experiments revealed that 20-hydroxyecodyson(20e)significantly induces the expression of the OfurGRX2 transcript,whereas juvenile hormone(JH)counteracts 20e effects.Adverse stress factors(including starvation,ultraviolet light,mechanical injury,Escherichia coli exposure,and high and low temperatures)dramatically induced OfurGRXGRX2 transcript expression,which confirmed for the first time that GRX2 play important roles in insecta during exposure to adverse environments.

硫化氢通过glutaredoxin-1调节氧化应激减轻急性阻塞性睡眠呼吸暂停诱发房颤的机制

目的探讨硫化氢(H_(2)S)减轻急性阻塞性睡眠呼吸暂停(OSA)诱发房颤的机制。方法硫氢化钠(NaHS)作为外源性H_(2)S供体,8~10周龄健康成年雄性SD大鼠24只,体质量320~360 g,随机分为对照组、OSA诱发房颤组、NaHS+OSA组和氯化镉+NaHS+OSA组,每组6只。按照既往文献构建OSA诱发房颤模型,实验结束后处死大鼠,留取左心耳组织。采用免疫荧光、ELISA法检测左心耳谷氧还蛋白-1的表达水平;采用硫代巴比妥酸法检测左心耳丙二醛(MDA)含量。结果与OSA组相比,NaHS+OSA组房颤诱发次数减少、房颤持续时间缩短(P<0.05);与对照组相比,OSA组左心耳谷氧还蛋白-1表达减少,MDA含量增加,应用NaHS后,NaHS+OSA组谷氧还蛋白-1表达水平较OSA组增加,MDA含量降低(P<0.01),在NaHS基础上应用谷氧还蛋白-1抑制剂氯化镉后,氯化镉+NaHS+OSA组MDA含量增加(P<0.01),H_(2)S减轻OSA诱发房颤的作用消失。结论外源性H_(2)S减轻急性OSA诱发房颤,可能是通过上调心肌细胞谷氧还蛋白-1表达从而减轻心肌细胞氧化应激。

Engineering human seleno-glutaredoxin containing consecutive rarecodons as an artificial glutathione peroxidase

The active center of human glutaredoxin(hGrx1)shares a common thioredoxin fold and specific affinity for substrate glutathione (GSH)with natural glutathione peroxidase(GPx).hGrx1 was redesigned to introduce the catalytic selenocysteine residue to imi- tate the function of antioxidant selenoenzyme GPx in vivo.The human hGrx1 scaffold is a good candidate for potential medical application compared with other animal-originated protein scaffolds.Two consecutive rare codons(AGG-AGG)in the open reading frame of hGrx1 mRNA encoding Arg26-Arg27 residues can reduce seleno-hGrx1 expression level significantly in the Cys auxotrophic Escherichia coli strain BL21cysE51.Therefore,we optimized the rare codons,which resulted in a remarkable in- crease of the expression level in the Cys auxotrophic cells,which may be sufficient for future medical production.The engineered artificial selenoenzyme displays high GPx catalytic activity,rivaling that of some natural GPx proteins.Kinetic analysis of the engineered seleno-hGrx1 showed a typical ping-pong kinetic mechanism;its catalytic properties are similar to those of some nat- urally occurring GPx proteins.

单增李斯特菌谷氧还蛋白调控氧化应激相关基因转录的研究

本实验室前期对单增李斯特菌(LM)谷氧还蛋白(Grx)转录组数据进行了分析,在此基础上为了对Grx调控细胞色素氧化酶等应激相关基因(lmo0722、qox A、qox B、gr)的转录及其作用机制研究,本研究将Δgrx与野生株EGD-e经4 mmol/L肼应激后,分别提取总RNA并反转录为cDNA作为模板,利用RT-q PCR检测Grx调控细胞色素氧化酶等应激相关基因转录情况,结果显示,Δgrx与野生株EGD-e相比,grx基因缺失引起qox B、qox A、gr、lmo0722等基因的转录水平显著上调(分别上调30、29、17和5.6倍)。利用李斯特菌穿梭质粒构建携带调控基因启动子序列的gfp报告质粒,电转化至野生株EGD-e和缺失株Δgrx感受态细胞中,获得含GFP的重组报告菌株。将这两种含GFP的重组报告菌液分别加入4 mmol/L肼后检测荧光强度,结果显示,EGD-e携带的GFP荧光数值显著低于缺失株Δgrx(P<0.01),进一步表明Grx参与调控上述应激相关基因的转录。将扩增的lmo0722、qox A、qox B和gr基因的启动子和Grx、Prf A和GAPDH重组蛋白混合,37℃孵育60 min后进行凝胶迁移试验(EMSA),结果显示,Grx和上述调控基因启动子不直接结合,提示Grx可能通过间接方式参与该调控过程。本研究首次证实LM Grx通过对氧化应激相关基因的转录调控进而在细菌抗氧化应激环境适应过程中发挥重要作用,为系统阐述重要食源性病原菌在环境适应中发挥作用的调控机制提供了科学参考。

miR-148a-3p靶向谷氧还蛋白5抑制肺癌细胞增殖迁移与侵袭

目的 探索miR-148a-3p对肺癌细胞增殖、迁移与侵袭的影响。方法 收集肺癌组织和配对癌旁组织以及肺癌细胞和正常肺上皮细胞株,RT-qPCR检测miR-148a-3p表达;Western blot和免疫组织化学检测谷氧还蛋白5(glutaredoxin 5,GLRX5)的表达。对A549细胞转染miR-148a-3p mimics和pcDNA-GLRX5后,分别用MTT、EdU、细胞划痕和Transwell实验检测细胞活性、细胞增殖、迁移和侵袭;Western blot和免疫荧光检测增殖细胞核抗原(proliferating cell nuclear antigen,PCNA)、Ki-67、基质金属蛋白酶-2(matrix metalloproteinase-2,MMP-2)和MMP-9表达。用生物信息学和荧光素酶测定法鉴定miR-148a-3p与GLRX5的靶向关系。结果 分别与癌旁组织或正常肺上皮细胞比较,肺癌组织和肺癌细胞中miR-148a-3p表达降低,GLRX5表达升高。转染miR-148a-3p mimics后,A549细胞活性、增殖、迁移和侵袭以及PCNA、Ki67、MMP-2和MMP-9表达均降低,而过表达GLRX5能显著逆转miR-148a-3p mimics的上述作用。GLRX5是miR-148a-3p的靶基因。结论 miR-148a-3p可通过靶向GLRX5来发挥对肺癌细胞增殖、迁移和侵袭的抑制作用。

番茄GRX基因家族的鉴定及表达分析

GRX基因家族是从原核生物到真核生物中普遍存在的一类巯基-二硫键氧化还原酶,在植物的生长发育、器官构建及逆境胁迫和激素信号应答中均发挥重要作用。本研究在番茄基因组范围内,利用生物信息学方法对番茄的GRX基因组家族的成员、分布及结构和功能等进行分析。预测结果显示,番茄GRX家族包含55个蛋白质,分为4个亚族,其中植物特有的CC亚族成员最多,有35个,其他GRX基因成员与拟南芥GRX家族具有相似分类。在番茄GRX结构域中包含12个重要的基序,主要分布在序列的N端,相同亚族中的GRX成员蛋白序列的氨基酸保守域构成基本一致,且各亚族成员的氨基酸保守域组成特异,表明这些基序的存在对GRX蛋白功能的执行是必需的。利用实时荧光定量PCR对番茄GRX基因的组织表达和胁迫响应分析,结果表明,GRX基因具有组织特异性表达差异,CC型在根和花中表达较高,在果实中表达较低;在盐、SA、ABA、高温和低温胁迫条件下,22个番茄GRX基因的表达模式被阐明;其中部分基因的表达水平被显著地诱导增加或者降低,很可能参与了调控番茄逆境胁迫条件下的防御应答反应。本研究结果将为番茄GRX家族基因的深入研究提供依据,为进一步解析GRX基因功能奠定基础。

重组人谷氧还蛋白1对小鼠脑缺血/再灌注损伤的保护作用

目的探讨重组人谷氧还蛋白1(rhGrx1)对小鼠局灶性脑缺血/再灌注损伤的保护作用及机制。方法线栓法制备小鼠脑缺血/再灌注模型,病理形态学方法证实模型建立成功。小鼠尾静脉注射rhGrx1(5mg·kg-1和10mg·kg-1)后,观察脑组织中乳酸脱氢酶(LDH)、超氧化物歧化酶(SOD)及蛋白质羰基含量的变化,Western blot检测小鼠脑组织中p38MAPK表达水平的变化。结果HE染色证实模型建立成功且提示rhGrx1可改善缺血/再灌注损伤所致的小鼠脑组织病理形态学变化;rhGrx1能增加小鼠脑组织LDH、SOD活性、降低蛋白质羰基的含量。与假手术组小鼠相比,缺血和再灌注时脑组织p38MAPK蛋白表达量明显增加,注射rhGrx1后p38MAPK蛋白表达被抑制。结论rh-Grx1对局灶性脑缺血/再灌注损伤小鼠有一定保护作用,其机制可能与抑制p38MAPK蛋白表达相关。

谷氧还蛋白系统及其对细胞氧化还原态势的调控

细胞内氧化还原调控主要是由谷氧还蛋白系统和硫氧还蛋白系统完成。谷氧还蛋白属于硫氧还蛋白超家族,广泛分布在各种生物体内。作为一种巯基转移酶,它能够催化巯基-二硫键交换反应或者还原蛋白质谷胱甘肽二硫化物,以维持胞内的氧化还原态势。谷氧蛋白系统参与氧化胁迫、蛋白修饰、信号转导、细胞调亡和细胞分化等多种生物过程。对其体内作用靶蛋白的研究,有助于阐明谷氧还蛋白在整个细胞氧化还原网络的重要调控作用。

Grx1抑制高糖诱导的H9c2细胞中Caspase-8/3和JNK/c-Jun凋亡通路的激活

谷氧还蛋白1(glutaredoxin 1,Grx1)作为一种重要的抗氧化剂,通过响应多种重要蛋白质的活动和功能调节细胞的关键过程.了解Grx1功能,对寻求糖尿病和心肌病等,以凋亡失调和氧化还原稳态改变为发病机制的疾病的新颖治疗策略至关重要.为研究Grx1对高糖诱导的大鼠心肌细胞凋亡的抑制作用及相关信号机制,本研究以高糖诱导大鼠心肌细胞H9c2建立高糖损伤模型,采用免疫印迹实验检测caspase-3、8、9蛋白活性片段的表达和凋亡信号蛋白JNK/c-Jun的磷酸化水平.结果显示,与正常对照组相比,高糖组caspase家族中,剪切的caspase-3、caspase-8、caspase-9相对含量均显著增多,JNK和c-Jun蛋白的磷酸化水平均显著上调.但给予外源性Grx1保护后,剪切的caspase-3和caspase-8相对含量均显著降低,JNK和c-Jun蛋白的磷酸化水平均显著下调.上述结果表明,高糖通过介导caspase-8/3和caspase-9/3凋亡通路,并激活凋亡相关信号通路JNK/c-Jun诱导H9c2心肌细胞凋亡.给予外源性Grx1保护后,可通过抑制caspase-8/3凋亡通路和JNK/c-Jun信号通路的激活,拮抗高糖诱导的心肌细胞凋亡.

谷氧还蛋白1调节高糖诱导的心肌细胞自噬

人谷氧还蛋白1（Grx1）在体内具有广泛的抗氧化、抗凋亡作用,与氧化应激损伤导致的糖尿病和心肌病等多种疾病的发病机制密切相关.研究表明,糖尿病心血管病与自噬调节异常密切相关,但糖尿病心血管病变时自噬水平如何调节才能够保护受损的心肌还尚未定论.为研究自噬在高糖诱导心肌细胞凋亡中的作用及其与Grx1的关系,以明确Grx1对高糖诱导的心肌细胞凋亡的抑制作用及相关机制,本研究以高糖诱导大鼠心肌细胞H9c2建立高糖损伤模型,采用氧化还原蛋白免疫印迹法检测蛋白质的氧化水平.免疫印迹检测活性caspase 3蛋白和自噬蛋白Beclin1和LC3以及抗凋亡蛋白Bcl-2的表达水平.研究发现,高糖可诱导蛋白质的氧化水平增加,而Grx1可拮抗高糖诱导的H9c2细胞中蛋白质的氧化.并且含血清的高糖（25和50 mmol/L）作用H9c2心肌细胞后,自噬蛋白Beclin 1表达水平在6-48 h显著上调.同时发现,活性caspase 3水平也呈时间依赖性表达上调,caspase 3和自噬蛋白表达水平的同趋势增加,说明升高的自噬水平与心肌细胞凋亡的调节有关.Grx1保护组的自噬蛋白及活性caspase 3表达水平均显著下调,Grx1抑制剂镉组可拮抗Grx1调节的自噬蛋白和凋亡蛋白水平,说明Grx 1通过抑制自噬及caspase 3水平抑制高糖诱导的心肌细胞凋亡.以上研究结果提示,通过提高Grx1/GSH抗氧化系统功能,调节氧化还原稳态,可以有效减少高糖诱导的心肌损伤,保护糖尿病心脏功能.

烟草谷氧还蛋白基因NbGRX1的克隆与表达特性分析

采用同源克隆及cDNA末端快速扩增法(RACE),从烟草中克隆到1个谷氧还蛋白基因(Grx),命名为NbGRX1。该基因全长1021bp,编码298个氨基酸,具有典型的Grx基因结构域。Real-timeRT-PCR分析表明,该基因能在烟草的根、茎、叶中表达,并且受低温、干旱和高盐诱导。

谷氧还蛋白和硫氧还蛋白对动物抗氧化应激生物学效应的研究进展

谷氧还蛋白和硫氧还蛋白分别是动物机体抗氧化酶系统和抗氧化非酶系统的重要成员,具有多种生物学作用,在调节机体的氧化还原反应、抑制细胞凋亡和肠道保护方面起着重要作用。本文结合谷氧还蛋白和硫氧还蛋白的结构与功能、抗氧化机制及抑制细胞凋亡的最新研究近况,就谷氧还蛋白和硫氧还蛋白对动物抗氧化应激生物学效应的研究进行了综述。

胰高血糖素样多肽-1拮抗2型糖尿病胰岛细胞凋亡损伤（英文）

胰高血糖素样多肽-1(glucogen-like peptide-1,GLP-1)在胰岛素分泌过程中扮演重要角色,并在改善β细胞功能方面有着令人瞩目的效应,但有关其作用机制尚需更深入研究。本研究探讨GLP-1对2型糖尿病(type 2 diabetes mellitus,T2DM)大鼠模型胰岛细胞损伤的影响,观察GLP-1在T2DM大鼠胰岛细胞凋亡损伤机制中所发挥的作用。HE染色结果发现,糖尿病大鼠胰岛损伤。ELISA结果表明,糖尿病患者和糖尿病大鼠血清中GLP-1表达水平上调。放射免疫结果表明,GLP-1和谷氧还蛋白1(Grx1)促进HIT-T 15细胞分泌胰岛素,Cd抑制胰岛素的分泌。免疫组化结果表明,糖尿病大鼠GLP-1加药处理后,各组与糖尿病组相比,药物提高了Grx1和胰岛素表达水平,降低了胰高血糖素表达水平,同时降低了活性胱天蛋白酶3(caspase-3)的表达。本研究结果提示,GLP-1在肥胖T2DM大鼠胰岛细胞凋亡中起保护作用,同时可调节胰岛素和胰高血糖素水平,其机制可能与Grx1相关。

血浆谷氧还蛋白水平与新诊断2型糖尿病患者颈动脉粥样硬化的相关性研究

目的探讨血浆谷氧还蛋白(Grx)水平与新诊断2型糖尿病(T2DM)患者颈动脉粥样硬化(CAS)的相关性。方法选取2016年1月~2016年5月于唐山市人民医院内分泌科就诊的新诊断T2DM患者100例作为研究对象。根据颈动脉超声检查结果将其分为CAS组(CAS组,n=52例)和非CAS组(NCAS组,n=48例)。同时从该院健康体检中心选取非糖尿病健康人群55例作为正常对照组(NC组,n=55例)。记录其年龄、性别、体重指数(BMI)、收缩压(SBP)、舒张压(DBP),收集其临床检验结果,包括空腹血糖(FPG)、糖化血红蛋白(HbA1C)、总胆固醇(TC)、三酰甘油(TG)、高密度脂蛋白胆固醇(HDL-C)、低密度脂蛋白胆固醇(LDL-C)、同型半胱氨酸(Hcy)及超敏C反应蛋白(hs-CRP)。采用酶联免疫吸附法(ELISA)检测血浆Grx水平。结果 3组间Grx水平比较结果显示,CAS组和NCAS组均高于NC组,CAS组高于NCAS组(均P<0.05);在T2DM患者中,Grx与HbA1c、hs-CRP均呈正相关(均P<0.05);在T2DM患者中,经Logistic回归分析发现,年龄(OR=1.225,P=0.021)、HbA1c(OR=1.754,P=0.016)、Grx(OR=1.556,P=0.009)均为其CAS发生的危险因素。结论新诊断T2DM患者血浆Grx与其CAS相关,提示Grx可能参与了CAS的发生及发展。