Effect of electroacupunture on gastric mucosal intestinal trefoil factor gene expression of stress-induced gastric mucosal injury in rats

AIM： To investigate electroacupunture（EA） at the acupoints of Stomach Meridian of Foot-Yangming（SMFY）, Gallbladder Meridian of Foot-Yangming（SMFY） on gastric mucosal intestinal trefoil factor （ITF） gene expression detection in stress-induced rats with gastric mucosal lesion, and to explore the regulatory mechanism and significance of EA-related gastric mucosal protective effect. METHODS： Forty rats were randomly divided into 4 groups： Blank group, Model group, Model group＋EA at acupoints of SMFY group（＂SMFY group＂）, and Model group＋EA at acupoints of GMFY group（GMFY group）. All rats （except blank group） were made model by water immersion and restraint stress （WRS）. Then the gastric mucosa tissue in each rat was taken off alter assessment of gastric mucosal lesion index（GUI）, and the expression of ITF mRNA of the tissues was detected by reverse transcdption-polymerase chain reaction（RT-PCR） method. RESULTS： Compared with Model group（S4.3± 1.34）, the GUI value in SMFY group （31±2.211 decreased significantly（P〈0.01）, so did that in GMFY group （39.8± 1.62, P〈0.05）, meanwhile GUI value in SMFY group was significantly lower than in GMFY group（P〈0.01）. Compared with Model group （0.65±0.01）, EA had a tendency to improve the expression of gastric mucosal ITFmRNA gene： such tendency existed in GMFY group （0.66±0.01） but with no signficant difference（P〉 0.05）, in SMFY group（0.76±0.01） with an extremely obvious difference （P〈0.01）, furthermore the expression in SMFY group was significantly higher than in GMFY group （P〈 0.01）.CONCLUSION： The gastric mucosal protective effect by EA at the acupoints of SMFY and GMFY was related to the expression variance of ITF, indicating certain meridian specificity exists, It could be one proof for the TCM theory ＂Relative pardcularity between SMFY and stomach＂.

Effects of Intestinal Trefoil Factor on Colonic Mucosa in Experimental Colitis of Rats

In order to investigate the protective effects of intestinal trefoil factor (ITF) on colonic mucosa in experimental colitis of rats, ITF was detected by RT-PCR and immunohistochemistry at different time points. Three days after colitis induction, rats were treated with either 0.9 % saline solution or rhITF. Pathological changes and the expression of iNOS mRNA, NO, MDA and SOD were measured respectively. It was found that ITF was mainly located in goblet cells, significantly higher in model group than in normal group (P<0.05). rhITF could increase the iNOS mRNA expression and NO contents, and there was statistically significant difference between rhITF group and model group (P<0.05). rhITF also caused an increase of MDA and a decrease of SOD, but there was no significant difference between two groups. These results indicated that ITF has apparent therapeutic effects in ulcerative colitis, which may be associated with iNOS and NO.

Pretreatment with intestinal trefoil factor alleviates stress-induced gastric mucosal damage via Akt signaling

BACKGROUND Stress-related gastric mucosal damage or ulcer remains an unsolved issue for critically ill patients.Stress ulcer prophylaxis has been part of routine intensive care,but uncertainty and controversy still exist.Co-secreted with mucins,intestinal trefoil factor(ITF)is reported to promote restitution and regeneration of intestinal mucosal epithelium,although the mechanism remains unknown.AIM To elucidate the protective effects of ITF on gastric mucosa and explore the possible mechanisms.METHODS We used a rat model of gastric mucosal damage induced by water immersion restraint stress and lipopolysaccharide-treated human gastric epithelial cell line to investigate the potential effects of ITF on damaged gastric mucosa both in vivo and in vitro.RESULTS ITF promoted the proliferation and migration and inhibited necrosis of gastric mucosal epithelia in vitro.It also preserved the integrity of gastric mucosa by upregulating expressions of occludin and zonula occludens-1.In the rat model,pretreatment with ITF ameliorated the gastric mucosal epithelial damage and facilitated mucosal repair.The protective effects of ITF were confirmed to be exerted via activation of Akt signaling,and the specific inhibitor of Akt signaling LY249002 reversed the protective effects.CONCLUSION ITF might be a promising candidate for prevention and treatment of stressinduced gastric mucosal damage,and further studies should be undertaken to verify its clinical feasibility.

Production of human intestinal trefoil factor in Pichia pastoris

Objective：To construct a Pichia pastoris （P. pastoris） expression vector of human intestinal trefoil factor （hITF） and study its expression and purification procedures. Methods：hITF gene encoding mature peptide was modified with a polybistidine tag sequence at the N-terminal, and then inserted into the P. pastoris expression vector pGAPZaA at the downstream of the s-mating factor signal. After gene sequencing, the recombinant pGAPZaA-hITF was transformed into the P. pastoris strain X-33 with lithium chloride, rhITF was induced to constitutively express in shake flask, and then analyzed with Tricine SDS-PAGEand Western blotting. The obtained rhITF was isolated from the cultured supernatants by ammonium sulfate precipitation, Ni-NTA affinity chromatography, and ultrafiltration. Results：The correctness and integrity of rhITF were identified by restriction digestion and gene sequencing, rhITF was successfully expressed to 50 mg/L as a secretive protein. After purification, the purity was above 95%. Tricine SDS-PAGE and Western-blot analysis showed that rhITF presented as a single band with a molecular weight of 10 kDa, a little larger than 7 879 Da as assayed by mass spectrometry analysis. Conclusion： hITF P. pastoris expression vector is successfully constructed and rhITF is expressed in P. pastoris at commercially relevant level. This research lays foundation for the further functional studying of hITF.

不同频次高压氧治疗对脑卒中早期患者神经功能和肠黏膜屏障功能及血清CIT IFABP ITF的影响

目的探究不同频次高压氧治疗对脑卒中早期患者神经功能、肠黏膜屏障功能及血清瓜氨酸(CIT)、肠型脂肪酸结合蛋白(IFABP)、肠三叶因子(ITF)的影响。方法将南京医科大学附属江宁医院收治的89例脑卒中患者随机分为对照组(29例,行常规药物治疗)、低频次组(30例,在对照组基础上给予低频高压氧治疗)、高频次组(30例,在对照组基础上给予高频高压氧治疗)。治疗前及治疗结束后4周评估3组患者神经功能、日常生活活动能力,同时检测3组患者肠黏膜屏障功能指标及血清CIT、IFABP、ITF水平,观察3组患者不良反应情况。结果治疗结束后4周,对照组、低频次组和高频次组患者NIHSS评分、内毒素(ET)、二胺氧化酶(DAO)、D-乳酸、IFABP、ITF水平均低于治疗前(P<0.05),MBI评分、CIT水平均高于治疗前(P<0.05)。与对照组相比,低频次组和高频次组患者NIHSS评分[分别为(6.23±2.05)分、(4.52±1.87)分]、ET[分别为(0.31±0.06)IU/mL、(0.21±0.05)IU/mL]、DAO[分别为(2.64±0.31)IU/mL、(1.71±0.18)IU/mL]、D-乳酸[分别为(0.16±0.04)mmol/L、(0.10±0.02)mmol/L]、IFABP[分别为(0.89±0.13)μg/L、(0.52±0.08)μg/L]、ITF[分别为(9.02±2.14)μg/L、(7.36±1.75)μg/L]水平更低(P<0.05),MBI评分[分别为(84.02±7.51)分、(90.89±5.42)分]、CIT[分别为(24.45±3.02)μmol/L、(31.42±3.31)μmol/L]水平更高(P<0.05)。与低频次组相比,高频次组患者NIHSS评分更低(P<0.05),MBI评分、CIT水平更高(P<0.05)。3组患者不良反应发生率比较差异无统计学意义(P>0.05)。结论早期对脑卒中患者实施高压氧治疗可明显改善患者神经功能、肠道黏膜屏障功能及胃肠功能,提高患者生活活动能力,安全性好,高频次高压氧的治疗效果更好。

血清ITF3、HMGB1水平对结直肠癌患者根治术后早期炎性肠梗阻的诊断价值

目的探讨血清肠三叶因子3(ITF3)和高迁移率族蛋白B1(HMGB1)水平对结直肠癌患者根治术后早期炎性肠梗阻(EPISBO)的诊断价值。方法选取2020年2月至2023年2月在我院确诊结直肠癌并进行手术的277例患者作为研究对象,选取同期在我院体检健康者277例为对照组。检测并分析两组患者血清ITF3、HMGB1水平。采用Logistic回归分析影响结直肠癌患者发生EPISBO的因素。采用Pearson分析EPISBO患者血清ITF3、HMGB1的相关性。受试者工作特征(ROC)曲线分析ITF3、HMGB1水平对结直肠癌患者EPISBO的诊断效能。结果研究组患者血清ITF3水平显著低于对照组(P<0.05),HMGB1水平显著高于对照组(P<0.05);Pearson等级相关分析显示,EPISBO患者血清ITF3、HMGB1水平呈现负相关性(r=-0.671,P<0.001)。Logistic回归结果显示,ITF3是结直肠癌患者术后发生EPISBO的独立保护因素(P<0.05),HMGB1是导致EPISBO的独立危险因素(P<0.05)。ROC曲线显示,血清ITF3、HMGB1联合应用诊断EPISBO的临床价值优于ITF3、HMGB1单独检测(Z_(二者联合-ITF3)=3.112、P=0.002,Z_(二者联合-HMGB1)=2.000、P=0.046)。结论结直肠癌术后发生EPISBO患者血清ITF3水平显著降低,HMGB1表达水平显著升高,二者对EPISBO的临床诊断预测具有重要意义。

hITF毕赤酵母表达载体的构建及分泌表达

目的构建hITF毕赤酵母分泌型表达载体,表达重组hITF,为功能研究奠定基础。方法通过PCR获得hITFcDNA片段,将目的基因插入酵母表达载体pGAPZαA分泌信号下游,得到重组载体pGAPZαA-hITF。BspHⅠ线性化后氯化锂转化进入X-33,Zeoc in筛选转化酵母菌,PCR鉴定目的基因。阳性转化子经摇瓶表达,取上清TCA沉淀后做Tric ine SDS-PAGE分析及W estern b lot检测。结果经测序及PCR证实,hITFcDNA准确插入酵母表达载体pGAPZαA中,氯化锂转化后,重组载体通过同源重组整合进入酵母基因组中。Tric ine SDS-PAGE分析证明hITF的分子量约为10×103,W estern b lot分析表明,表达蛋白具有良好的抗原性和特异性。结论成功构建出酵母表达载体pGAPZαA-hITF,获得重组hITF,为深入研究hITF奠定了基础。

断奶仔猪血清及肠道肠三叶因子ITF水平与腹泻的关系研究

观察仔猪断奶后一周的腹泻情况,比较民猪和长白猪的腹泻程度。用ELISA方法检测断奶仔猪血清和肠道肠三叶因子(Intestinal trefoil factor,ITF)浓度,分析断奶后ITF水平变化与仔猪断奶腹泻的关系。结果表明,断奶后一周内,民猪腹泻率、腹泻频率和腹泻指数均小于长白,提示民猪比长白具有更好的抵抗腹泻的能力。断奶后仔猪血清和肠道ITF水平发生了显著变化,健康组仔猪血清ITF含量极显著上调(P<0.01),腹泻组肠道ITF水平在空肠和盲肠显著上调(P<0.05),而健康组肠道ITF水平相对较稳定,提示ITF与仔猪断奶腹泻有重要关系,断奶仔猪维持肠道较稳定的ITF水平,是保证肠道健康,减少腹泻发生的重要生理基础。

人小肠三叶因子(hITF)基因在生菜中的整合与表达

用根癌土壤杆菌 (Agrobacteriumtumefaciens (SmithetTownsend )Conn)介导的叶盘法 ,将人小肠三叶因子(hITF)导入生菜 (LactucasativaL .)中 ,在含有除草剂的培养基上筛选 ,获得抗性植株。通过PCR和Southern印迹分析证明 ,hITFcDNA已整合到生菜基因组中。Western印迹分析证明hITF在生菜中的表达。ELISA检测表明 ,hITF在生菜新鲜叶片中的表达量为 2 0 0～ 3 0 0ng/g ,最高达 70 0ng/g ,约占总可溶性蛋白的 0 .1%。

隔药灸与电针对溃疡性结肠炎大鼠结肠黏膜ITF、IL-8表达的影响

目的研究隔药灸与电针大肠下合穴上巨虚对溃疡性结肠炎(UC)大鼠结肠黏膜肠三叶因子(ITF)、白介素8(IL-8)表达的调节作用。方法将大鼠随机分为正常组、模型组、隔药灸组、电针组。采用免疫法加局部刺激制备UC大鼠模型,隔药灸组、电针组选取上巨虚穴,分别进行隔药灸、电针治疗,连续治疗14次。治疗后记录大鼠症状体征变化;光镜下观察结肠形态学改变;采用免疫组化观察ITF、IL-8的表达变化。结果溃疡性结肠炎大鼠结肠黏膜ITF表达显著低于正常组(P<0.01),IL-8表达明显高于正常组(P<0.05);隔药灸组、电针组治疗后,大鼠体重增加,腹泻、脓血便等症状体征和结肠形态学损伤均明显改善;结肠黏膜ITF表达均较模型组显著增强(P<0.01),IL-8表达均较模型组明显降低(P<0.05)。结论UC大鼠结肠黏膜ITF表达明显降低,IL-8表达显著增高,隔药灸、电针上巨虚穴均能调节ITF和IL-8的异常表达。

PAF对肠上皮细胞紧密连接的影响及ITF的保护作用

目的:探讨血小板活化因子(PAF)是否会引起肠黏膜屏障的破坏以及这种破坏机制是否与紧密连接相关,并观察肠三叶因子(ITF)的保护作用.方法:培养人结肠腺癌细胞株Caco-2,分别设正常对照组:不加刺激物及干预因素;实验组:加入PAF,终浓度分别为50 ng/L、100 ng/L和200 ng/L;ITF预防组:先加入ITF0.3 g/L,30 min后加入PAF 100 ng/L;ITF治疗组:先加入PAF 100 ng/L,30 min后加入ITF0.3 g/L,24 h后进行实验.MTT比色法检测细胞活力;测定跨上皮电阻TER和荧光黄的透过量反映肠上皮细胞单层通透性;RT-PCR法检测紧密连接蛋白ZO-1和Occludin mRNA表达的变化;免疫荧光染色观察紧密连接蛋白ZO-1和Occludin的形态学.结果:PAF未影响到细胞的增殖和细胞活力.各浓度PAF作用24 h后,细胞单层通透性增加,跨上皮电阻(TER)下降,荧光黄透过增加.ITF治疗组及预防组TER下降值较模型组明显降低(122.2±14.7,100.3±10.9 vs 210.3±26.4,P<0.05),荧光黄透过量减少(10226.1±556.2,9711.2±364.9 vs 11601.2±693.5,P<0.05),预防组作用更明显.PAF作用后,ZO-1和Occludin mRNA表达均有下降,以100 ng/L组改变最为明显,ITF预防组较之表达增加(1.28±0.06 vs 1.07±0.05,1.13±0.07 vs 0.81±0.06,P<0.05),ITF治疗组改变不明显.免疫荧光染色发现ZO-1和Occludin主要分布在细胞内近胞膜处.PAF作用后,ZO-1及Occludin形态学改变,预防性给予ITF后,可明显减轻这种改变.结论:PAF可引起肠黏膜屏障破坏,其机制可能和紧密连接蛋白的破坏相关;ITF可以通过改变紧密连接蛋白的表达而部分恢复肠黏膜正常通透性,起到保护作用.

止痛如神汤对溃疡性结肠炎大鼠结肠黏膜ITF基因表达的影响

目的:观察止痛如神汤对溃疡性结肠炎的作用机制。方法:将40只健康雄性SD大鼠随机分为4组:正常组、模型组、奥沙拉嗪组(西药组)和止痛如神汤组(中药组),每组10只。除正常组外,其余3组均采用TNBS法制备UC大鼠动物模型。造模成功后开始药物干预,持续用药3周后分别取各组大鼠结肠组织,采用免疫组化法检测UC大鼠结肠黏膜ITF的含量。结果:经免疫组织化学法检测,模型组大鼠结肠黏膜ITF棕黄色阳性细胞表达较正常组明显减少,其阳性细胞的数目及平均光密度值皆明显下降,与正常组比较有明显统计学意义(P<0.01)。中药组和西药组大鼠在结肠黏膜棕黄色阳性细胞表达较模型组显著升高,其差异有统计学意义(P<0.05)。结论:止痛如神汤有促进TNBS法UC大鼠模型结肠黏膜ITF基因表达上调的作用,这可能是其抗UC作用的机理之一。

含hITF基因cDNA的腺病毒载体的构建及其感染肠上皮细胞的研究

目的构建含有人肠三叶因子基因cDNA的腺病毒载体,并观察其对肠上皮细胞的感染能力。方法利用PCR技术扩增hITF基因cDNA全长序列,测序后亚克隆至腺病毒穿梭质粒,转化至含腺病毒骨架质粒pAdEasy-1大肠杆菌株BJ5183感受态细胞中进行同源重组,内切酶PmeⅠ线性化后转染HEK293细胞进行病毒包装及扩增,并进行滴度测定。将重组腺病毒感染肠上皮细胞(HT-29),荧光显微镜观察感染效果。结果成功构建出重组穿梭质粒pAdTrack-CMV-hITF,PmeⅠ线性化后与骨架质粒pAdEasy-1同源重组,PacⅠ酶切鉴定后命名为Ad-hITF;重组腺病毒载体在HEK293细胞中包装,获得重组腺病毒颗粒;根据Karbers公式计算病毒颗粒滴度为2×109 pfu/mL;重组腺病毒可以感染肠上皮细胞(HT-29),感染效率较高。结论成功构建含hITF基因cDNA的重组腺病毒载体并获得大量子代重组腺病毒,为腺病毒介导hITF基因治疗的应用打下基础。

ITF通过JAK-STAT3途径上调自身启动子的活性

目的:研究肠三叶因子(intestinal trefoil factor,ITF)对自身启动子活性的影响及Janus激酶/信号转导和转录激活因子(Janus kinase/signal transducers and activators of transcription,JAK/STAT)信号通路对其的调控作用。方法:以人全血基因组DNA为模板,PCR获取ITF基因5'侧翼序列,插入p GL3-Basic载体,构建ITF启动子重组载体;以不同浓度的ITF刺激,检测双荧光素酶的活性;运用JAK-STAT3通路特异性抑制剂AG490阻断JAKSTAT3信号通路,观察AG490对ITF启动子活性的影响。结果:酶切和直接测序法证实包含ITF启动子的重组质粒构建成功;瞬时转染实验显示,ITF能显著提高ITF启动子的活性(P<0.05);加入AG490后ITF启动子活性显著下降(P<0.05)。结论:ITF通过JAK-STAT3途径上调自身启动子的活性。

含hITF启动子的荧光素酶报告质粒的构建及活性检测

目的构建含有人肠三叶因子(intestinal trefoil factor,hITF)启动子的荧光素酶表达载体,并检测启动子活性。方法采用PCR技术从LS-174T细胞基因组DNA中扩增出长约2.5kb的含hITF基因启动子片段(-2331/+53),而后在此基础上构建了10个不同长度的启动子序列至pGL-3basic荧光素酶表达载体,然后将这些重组质粒转染HEK-293细胞并在48h后检测其荧光素酶活性。结果插入的hITF启动子片段测序结果显示正确,-500/+53,-400/+53和-300/+53片段活性介于0.023～0.026之间,-200/+53,-100/+53和-50/+53活性介于0.0032～0.0042之间,明确了最小活性功能域位于-300/+53区域,-300/-200区域对hITF转录起始起关键性作用。结论成功构建了含hITF启动子的萤火虫荧光素酶报告基因质粒,鉴定出人肠三叶因子(hITF)启动子活性位于-300/-200区域。

转人小肠三叶因子侧耳中hITF的表达及在大鼠体内生物活性研究

将人小肠三叶因子(hITF)用原生质体法导入糙皮侧耳(Pleurotusostreatus)中,检测表明,hITF在侧耳新鲜菌丝体中的表达量约为 10 0 0～ 2 0 0 0ng/g,最高约达 2 2 5 0ng/g.体内生物学活性研究证实,口服转hITF侧耳可有效地防止乙醇诱导的大鼠胃溃疡。

从脑肠轴探讨黄芪建中汤对胃溃疡大鼠肝细胞生长因子及ERK1/2和TFF3蛋白表达的影响

目的观察黄芪建中汤对脾胃虚寒型胃溃疡大鼠胃组织中肝细胞生长因子(HGF)及下丘脑和海马区中磷酸化细胞外信号调节激酶1/2(p-ERK1/2)及肠三叶因子3(TFF3)蛋白表达的影响,探究黄芪建中汤治疗脾胃虚寒型胃溃疡的作用及可能机制。方法用随机数字表法将60只大鼠分为正常组、模型组、奥美拉唑组和黄芪建中汤组,每组15只。正常组隔日蒸馏水灌胃,每日不限饮食;其余组大鼠先以小承气汤结合饥饱失常法复制脾胃虚寒证模型,实验第11天采用冰醋酸法建立胃溃疡模型。之后模型组继续隔日上午给予小承气汤并当日禁食,次日恢复饮食,共持续20 d;奥美拉唑组和黄芪建中汤组大鼠除同模型组的每日处理外,每日下午分别给予4.2 mg/(kg·d)奥美拉唑和6.8 g/(kg·d)黄芪建中汤灌胃;正常组隔日上午及每日下午给予蒸馏水灌胃。实验结束后摘取各组大鼠胃,记录溃疡大小并计算胃溃疡指数,HE染色观察胃组织病理形态,免疫组化染色检测胃组织中HGF及下丘脑和海马区中p-ERK1/2、TFF3蛋白阳性表达情况。结果正常组大鼠胃黏膜正常,未见溃疡点及糜烂斑等;模型组大鼠胃黏膜皱襞存在中断,有点状溃疡、糜烂及大量炎性细胞浸润;黄芪建中汤组与奥美拉唑组胃黏膜损伤较模型组轻,有少量炎性细胞浸润,未见明显溃疡。奥美拉唑组和黄芪建中汤组大鼠的胃溃疡指数均明显低于模型组(P均<0.05),胃组织中HGF及下丘脑和海马区中p-ERK1/2、TFF3蛋白表达平均光密度均明显高于模型组(P均<0.05)。结论黄芪建中汤能促进脾胃虚寒型胃溃疡大鼠溃疡愈合,上调HGF、ERK1/2及TFF3的表达可能是其基于脑肠轴治疗脾胃虚寒型胃溃疡的作用机制之一。

肠型脂肪酸结合蛋白、Toll样受体4、肠三叶因子与脑卒中患者胃肠功能障碍的相关性研究

目的分析肠型脂肪酸结合蛋白(intestinal fatty acid-binding protein,IFABP)、Toll样受体4(Toll-like receptor 4,TLR4)、肠三叶因子(intestinal trefoil factor,ITF)与脑卒中患者胃肠功能障碍的相关性。方法根据患者入院7d内是否出现胃肠功能障碍将68例脑卒中患者分为对照组(无胃肠功能障碍,n=41)和观察组(出现胃肠功能障碍,n=27)。比较两组美国国立卫生研究院卒中量表(National Institutes of Health Stroke Scale,NIHSS)评分以及IFABP、TLR4、ITF水平。统计两组患者预后良好率;使用受试者工作特征曲线(receiver operating characteristic curve,ROC)分析IFABP、TLR4、ITF水平在预估脑卒中患者胃肠功能障碍发生和不良预后的价值。结果与对照组比较,观察组NIHSS评分以及IFABP、TLR4、ITF水平均较高(P<0.05)。观察组预后良好率(55.56%)较对照组(78.05%)低(P<0.05);IFABP、TLR4、ITF水平预测脑卒中患者胃肠功能障碍发生的最佳临界值为IFABP≥367.85μg/L、TLR4≥3.78ng/ml、ITF≥14.40μg/L,此时曲线下面积为0.851、0.838、0.744(P<0.05),灵敏度为77.78%、70.37%、77.78%,特异度为92.68%、92.68%、75.61%。IFABP、TLR4、ITF水平预测脑卒中患者不良预后的最佳临界值为IFABP≥336.10μg/L、TLR4≥3.05ng/ml、ITF≥15.95μg/L,此时曲线下面积为0.914、0.925、0.930(P<0.05),灵敏度为100.00%、100.00%、76.19%,特异度为70.21%、65.96%、95.74%。结论存在胃肠功能障碍的脑卒中患者NIHSS评分以及IFABP、TLR4、ITF水平均较高,且不良预后发生风险较高,检测脑卒中患者IFABP、TLR4、ITF水平可了解胃肠功能障碍发生风险和不良预后发生风险。

肠三叶因子在大鼠肠道中表达的实验研究

目的 研究肠三叶因子 (ITF)及其mRNA在大鼠肠道的分布规律。方法 采用原位杂交、免疫组化等手段观察了ITF及ITFmRNA在大鼠肠道的表达并使用高效液相色谱仪检测了不同肠段ITF的含量。结果 从十二指肠至结肠均有ITF及ITFmRNA表达 ,主要分布于肠绒毛杯状细胞 ,其中ITFmRNA仅在杯状细胞的基底和边缘表达 ,其它区域的杯状细胞则呈ITFmRNA阴性反应 ,同时发现部分其它部位的肠上皮细胞中亦有少量ITF及ITFmRNA表达。ITF定量分析显示 ,整个肠道中以十二指肠含量最高 ,空回肠次之 ,结肠含量较低 ,各段小肠中ITF含量差异不显著 (P >0 .0 5 ) ,但都明显高于结肠 (P <0 .0 1)。结论 杯状细胞是合成ITF的主要场所 ,ITF在肠道分布的差异可能同各肠段分泌的粘液性质不同有关。

肠三叶因子在内毒素致幼鼠肠损伤中的作用及意义

目的探讨内毒素(LPS)致幼鼠肠损伤中二胺氧化酶(DAO)及肿瘤坏死因子(TNF-α)的变化及基因重组肠三叶因子(rITF)的保护作用,为临床治疗提供实验依据。方法Wistar幼鼠10日龄96只分为3组,A组:生理盐水对照组;B组:LPS组;C组:LPS+rITF组,每组32只。以生理盐水(1mL/kg),EcoliO55:B5(1mL/kg)、rITF(0.1mL/只、配制浓度5g/L)腹腔注射后2,6,24,72h断头处死动物,取动静脉混合血,测血DAO活性。留取肠组织,免疫组化法检测TNF-α蛋白含量,PCR法检测TNF-αmRNA表达。同时作电镜观测肠组织超微结构变化。结果B组血浆DAO活性自LPS作用后2h即开始升高,至6h达到最高值,较A组差异有显著性(1.519±0.13U/Lvs1.081±0.04U/L,P<0.01),72h仍持续高值;C组血浆DAO活性较B组明显下降(P<0.01或P<0.05);与A组6h比较差异有显著性(P<0.01),其余各时间点差异无显著性(P>0.05);B组TNF-α积分光密度含量明显高于A组,以LPS作用后6h达高峰(37247.64±3387.59vs6191.02±482.32,P<0.01),C组TNF-α含量较B组明显降低,但仍高于A组(P<0.01);TNF-αmRNA在A组各时间点有微弱的表达,在B组各时间点表达明显增强,较A组差异显著(P<0.01);而C组各时间点表达明显减少,较B组差异显著(P<0.01或P<0.05)。电镜下肠组织超微结构:A组正常,B组变化明显,C组变化较B组减轻。结论ITF可降低血浆DAO活性,抑制肠组织TNF-αmRNA及蛋白表达,减轻LPS所致幼鼠肠损伤,发挥保护作用。