Growth induction of hepatic stimulator substance in hepatocytes through its regulation on EGF receptors

The cytosolic liver-specific growth factor-hepatic stimulator substance (HSS) has been shown to be able to amplify the rat hepatocyte proliferation responded to EGF. In order to get more insight into the mechanism, the regulatory effect of HSS on EGF-receptor(EGF-R) and the receptor phosphorylation at molecular level was studied. HSS partially purified from weanling rat liver was given to cultured hepatocytes and its influence on EGF-R specific binding and internalization as well as mRNA expression were investigated. The results showed that preincubation of hepatocytes with HSS could lead to an increase in [125I]-EGF binding to its receptors and inhibit EGFinduced receptor down-regulation. Furthermore, the overexpression of EGF-R mRNA stimulated by HSS was seen during 2-12 h after the incubation. Additionally, it was demonstrated with human hepatoma sMMC-7721 cells in Western blot that the EGF-R expression and the receptor autophosphorylation were increased with dose/timedependency after HSS treatment. These results strongly suggest that the mechanism of HSS action on hepatocyte growth might be related to its modulation on EGF-R and receptor-mediated signaling transduction.

Purification and Characterization of Hepatocyte Regeneration Stimulatory Factor from Shark Liver

Aim To purify hepatocyte regeneration stimulatory factor from shark liver and research its molecular feature and activity. Methods and Results Hepatocyte regeneration stimulatory factor (sHRSF) was isolated from healthy shark livers and separated by homogenization, freezing melting, heat treating, centrifugation, and ultrafiltration. HRSF activity was found mainly in the subfraction of molecular weight less than 30 000 daltons. This crude ultrafiltrate was further purified successively by DEAE Sepharose fast flow chromatography, FPLC Resource 30Q, Resource Q and Mono Q chromatography. A single band was displayed on sodium dodecyl sulfate polyacrylamide gel electrophoresis, which corresponds to molecular weight of 14 600 daltons. The characteristic absorption was obtained at the wavelength 276 nm. The isoelectric point was about 5 1. It contained 18 amino acids and the 15 N terminal amino acid residues were LVGPIGAVGPAGKDG. It had a significant activity in stimulating liver to regenerate. Conclusion We obtained an unknown new active protein, that is hepatocyte regeneration stimulatory factor from shark liver (sHRSF).

Insights on augmenter of liver regeneration cloning and function

Hepatic stimulator substance （HSS） has been referred to as a liver-specific but species non-specific growth factor. Gradient purification and sequence analysis of HSS protein indicated that it contained the augmenter of liver regeneration （ALR）, also known as hepatopoietin （HPO）. ALR, acting as a hepatotrophic growth factor, specifically stimulated proliferation of cultured hepatocytes as well as hepatoma cells in vitro, promoted liver regeneration and recovery of damaged hepatocytes and rescued acute hepatic failure in vivo. ALR belongs to the new Erv1/Alr protein family, members of which are found in lower and higher eukaryotes from yeast to man and even in some double-stranded DNA viruses. The present review article focuses on the molecular biology of ALR, examining the ALR gene and its expression from yeast to man and the biological function of ALR protein. ALR protein seems to be non-liver-specific as was previously believed, increasing the necessity to extend research on mammalian ALR protein in different tissues, organs and developmental stages in conditions of normal and abnormal cellular growth.

Changes in growth factor and cytokine expression in biliary obstructed rat liver and their relationship with delayed liver regeneration after partial hepatectomy

AIM： To study the effects of obstructive jaundice on liver regeneration after partial hepatectomy. METHODS： Hepatocyte growth factor （HGF）, its receptor, c-Met, vascular endothelial growth factor （VEGF） and transforming growth factor-β1 （TGF-β1） mRNA expression in both liver tissue and isolated liver cells were investigated after biliary obstruction （BO） by quantitative reverse-transcription polymerase chain reaction （RT-PCR） using a LightCycler. Immunohistochemical staining for desmin and e-smooth muscle actin （α-SNA） was also studied. Regenerating liver weight and proliferating cell nuclear antigen （PCNA） labeling index, and growth factor expression were then evaluated after 70% hepatectomy with concomitant internal bUiary drainage in BO rats or sham-operated rats. RESULTS： Hepatic TGF-β1 mRNA levels increased significantly 14 days after BO, and further increased with duration of cholestasis. Meanwhile, HGF and VEGF tended to increase, but was not significant. In cell isolates, TGF-β1 mRNA was found mainly in the hepatic stellate cell （HSC） fraction. Immunohistochemical studies revealed an increased number of HSCs （desmin-positive cells） and activated HSCs （α-SMA-positive cells） in portal areas after BO. In a hepatectomy model, liver regeneration was delayed in BO rats, as compared to sham-operated rats. TGF-β1 mRNA was significantly up-regulated up to 48 h after hepatectomy, and the earlier HGF mRNA peak was lost in BO rats. CONCLUSION： BO induces HSCs proliferation and activation, leading to up-regulation of TGF-β1 mRNA and suppression of HGF mRNA in livers. These altered expression patterns may be strongly involved in delayed liver regeneration after hepatectomy with obstructive jaundice.

Partial isolation and identification of hepatic stimulator substance mRNA extracted from human fetal liver

IM To partially isolate and identify hepatic stimulator substance mRNA from human fetal liver tissues.METHODS The poly (A)mRNA was extracted from human fetal liver tissues of 4-5 month gestation, fractionated by size on sucrose gradient centrifugation, translated into protein from each fraction in vitro and then its products were tested for HSS activity.RESULTS Twentytwo 500μg total RNA was obtained from human fetal liver tissues and pooled. mRNA of 420μg was yielded, processed by oligo(dT)cellulose column chromatography, then was sizefractionated by ultracentrifution on a continuous sucrose density gradient (5%-25%), and separated into 18 fractions. Translated products of mRNA in fraction 8 and 9 could produce a twofold increase in the incorporation of 3HTdR into DNA of SMMC7721 hepatoma cells and in a heatresistant and organspecific way.CONCLUSION The partially purified HSS mRNA was obtained and this would facilitate the cloning of HSS using expression vectors.

Human augmenter of liver regeneration: molecular cloning, biological activity and roles in liver regeneration

The complete amino acid sequence of human augmenter of liver regeneration (hALR) was reported by deduction from nucleotide sequence of its complementary DNA . The cDNA for hALR was isolated by screening a human fetal liver cDNA library and the sequencing of this insert revealed an open reading frame encoding a protein with 125aa and highly homologous (87% ) with rat ALR encoding sequence. The recombinant hALR expressed from its cDNA in transient expression experiments in cos-7 cells could stimulate DNA synthesis of HTC hepatoma cell in the dose-dependent and heat-resistant way. Northern blot analysis with rat ALR cDNA as probe confirmed that ALR mRNA was expressed in the normal rat liver at low level and that dramatically increased in the regenerating liver after partial hepatectomied rat. This size of hALR mRNA is 1.4 kb long and expressed in human fetal liver, kidney and testis. These findings indicated that liver itself may be the resource of ALR and suggested that ALR seems to be an im-portant paracrined regulator of liver regeneration.

Immunohistochemical study of hepatic oval cells in human chronic viral hepatitis

AIM: To detect immunohistochemically the presence of oval cells in chronic viral hepatitis with antibody against c-kit. METHODS: We detected oval cells in paraffin embedded liver sections of 3 normal controls and 26 liver samples from patients with chronic viral hepatitis, using immunohistochemistry with antibodies against c-kit, piclass glutathione S-transferase (pi-GST) and cytokeratins 19 (CK19). RESULTS: Oval cells were not observed in normal livers. In chronic viral hepatitis, hepatic oval cells were located predominantly in the periportal region and fibrosis septa,characterized by an ovoid nucleus, small size,and scant cytoplasm. Antibody against stem cell factor receptor, c-kit, had higher sensitivity and specificity than pi-GST and CK19. About 50%-70% of c-kit positive oval cells were stained positively for either pi-GST or CK19. CONCLUSION: Oval cells are frequently detected in human livers with chronic viral hepatitis, suggesting that oval cell proliferation is associated with the liver regeneration in this condition.

人脐带间充质干细胞来源的细胞外囊泡增强纤维化肝脏再生能力

目的探讨人脐带间充质干细胞来源的细胞外囊泡(hUC-MSC-EV)在纤维化肝脏再生中的作用。方法将C57BL/6小鼠随机分为正常肝脏70%肝切除组(Oil+PHx组)、肝纤维化70%肝切除组(CCl_(4)+PHx组)、肝纤维化70%肝切除+间充质干细胞来源的细胞外囊泡(MSC-EV)治疗组(CCl_(4)+PHx+MSC-EV组),每组8只。将LX-2细胞分为磷酸盐缓冲液(PBS)组、转化生长因子(TGF)-β组、TGF-β+MSC-EV组。检测各组小鼠肝部分切除术后丙氨酸转氨酶(ALT)、天冬氨酸转氨酶(AST)、乳酸脱氢酶(LDH)水平,分析各组小鼠肝组织纤维化及增殖相关指标的表达情况。检测各组LX-2细胞表皮细胞生长因子(EGF)、成纤维母细胞生长因子(FGF)、血管内皮生长因子(VEGF)、肝细胞生长因子(HGF)信使RNA(mRNA)的表达水平。观察对小鼠肝脏HGF表达的影响。结果与Oil+PHx组比较,CCl_(4)+PHx组小鼠血清AST、ALT、LDH水平升高,纤维化程度较高,天狼星红及α-平滑肌肌动蛋白(α-SMA)染色阳性区域面积增大,α-SMA蛋白表达水平升高;与CCl_(4)+PHx组比较,CCl_(4)+PHx+MSC-EV组小鼠血清AST、ALT、LDH水平下降,纤维化程度较轻,天狼星红及α-SMA染色阳性区域面积缩小,α-SMA蛋白表达水平下降,差异均有统计学意义(均为P<0.05)。与Oil+PHx组比较,CCl_(4)+PHx组Ki67、增殖细胞核抗原(PCNA)蛋白表达水平降低;与CCl_(4)+PHx组比较,CCl_(4)+PHx+MSC-EV组Ki67、PCNA蛋白表达水平升高,差异均有统计学意义(均为P<0.05)。与PBS组比较,TGF-β组LX-2细胞内CollagenⅠmRNA表达水平升高,α-SMA蛋白表达水平升高,HGF蛋白表达水平下降;与TGF-β组比较,TGF-β+MSC-EV组LX-2细胞内CollagenⅠmRNA表达水平下降,HGF mRNA和蛋白表达水平升高,α-SMA蛋白表达水平降低,差异均有统计学意义(均为P<0.05)。CCl_(4)+PHx组HGF蛋白表达水平较Oil+PHx组下降,但差异无统计学意义(P>0.05);CCl_(4)+PHx+MSC-EV组HGF蛋白表达水平较CCl_(4)+PHx组上升,差异有统计学意义(P<0.05)。结论纤维化肝脏再生能力较正常肝脏减弱,hUC-MSC-EV可以减轻肝纤维化,并可能通过促进活化的肝星状细胞分泌HGF,有效改善纤维化肝脏的肝再生能力。

重症酒精性肝炎治疗进展

酒精性肝病是最常见的肝病之一,近年来患病率呈上升趋势。重症酒精性肝炎是酒精性肝病最严重的一种,其死亡原因与肝衰竭和多器官功能衰竭的发展相关,预后差,显著增加医疗负担。目前缺乏针对重症酒精性肝炎患者特异有效的治疗意见,常用的糖皮质激素治疗效果有限,对糖皮质激素无应答的患者预后更差,1年内死亡率极高。本文以重症酒精性肝炎的危险因素及发病机制为线索,总结了几种重症酒精性肝炎治疗方案及其效果,以期指导临床医生做出更佳的临床决策,延缓患者疾病进展,减轻社会医疗负担。

肝细胞移植的研究进展

肝脏是维持人体代谢和解毒等功能的重要器官。当出现急慢性肝衰竭或基因缺陷,肝功能受损无法满足机体所需时,肝移植常作为治疗首选。然而,由于肝源短缺等问题,肝移植的应用受到限制,人们开始发展与肝细胞移植相关的治疗方法。肝细胞移植的可行性已在多种动物模型中得到证实,用于促进肝再生或减少肝脏纤维化的各种类型自体细胞移植的临床试验也已开始实践。本文重点回顾了肝细胞移植的主要临床适应证、移植细胞的来源选择及肝细胞移植的技术问题,以期推进肝细胞移植相关研究,使肝细胞移植在临床治疗中取得广泛收益,为供体器官短缺提供切实可行的解决策略。

ERK1/2 contributes negative regulation to STAT3 activity in HSS-transfected HepG2 cells

Signal transducer and activator of transcription 3 (STAT3) is a recently characterized transcription factor which is essential to liver regeneration. We have previously reported that hepatic stimulator substance (HSS), a novel growthpromoting substance, phosphorylated the epidermal growth factor (EGF) receptors and activated downstream RasMAP kinase (extracellular signal-regulated kinases, ERK1/2) cascade. However, whether HSS signal is related to STAT3pathway remains unclear. The present study is aiming to explore the regulatory effect of activation of ERK1/2 evoked by HSS on STAT3 phosphorylation and STAT3 signaling. Human hepatoma cell line HepG2 was stably transfected with HSS cDNA and HSS expression was measured by Northern blot. The results showed that the transfection of HSS into HepG2 resulted in remarkable increase in cellular proliferation as compared with the non-transfected cells, and it was further proved that the cellular proliferation in the HSS-transfected cells was related to ERK1/2 activation. Treatment of the cells with 50 μM of PD98059, an ERK1/2 specific upstream inhibitor, resulted in ERK1/2 inactivation completely.Inhibition of ERK1/2 allowed the tyrosine of STAT3 to be phosphorylated in a dose-dependent manner to PD98059.Furthermore, transient transfection of STAT3 mutant (STAT3S727A) into HSS-bearing cells could remarkably reverse the inhibitory effect of ERK1/2 on STAT3 phosphorylation. Based upon these results, it is concluded that ERK1/2negatively modulates STAT3 phosphorylation and this function is dependent on residual serine-727 (S727) of STAT3.

肝再生增强因子的cDNA克隆、表达及表达产物的生物活性研究

以肝部分切除后再生肝组织为起始材料，利用RT-PCR扩增出大鼠肝再生增强因子（ALR），亚克隆于pGEM-T载体，核苷酸序列测定证实为大鼠ALR；将ALRcDNA亚克隆于pBV220质粒，构建了原核表达栽体，并获高效表达菌株，特异表达蛋白占细菌总蛋白的15％，原核表达的ALR在体外缺乏促进大鼠原代培养肝细胞及SMMC-7721肝癌细胞DNA合成的活性，但在体内1／3肝部分切除模型中可刺激肝细胞DNA合成；ALR在生物学活性方面与肝脏刺激物（HSS）存在一定差别，ALR和HSS应是两种不同的活性因子．ALR还具有促肝损伤修复的作用，对其深入研究可能为临床治疗严重肝病提供有效的药物.

肝再生增强因子研究进展

肝再生增强因子是新近克隆的蛋白质因子 ,能特异地刺激肝源细胞的增殖 ,并对CCl4 所引起的急性肝衰竭有救治作用。本文综述了肝再生增强因子的发现、基因克隆及组织分布等。目前已开始了该因子的基因工程产品研制 。

肝细胞刺激因子对肝癌细胞和大鼠肝细胞增生作用的研究

目的探讨肝细胞刺激因子 (HSS)对正常大鼠肝细胞和人肝癌细胞的作用特点。方法应用自制的HSS分别与正常大鼠肝脏细胞和人传代肝癌细胞共同培养不同时间 ,以促进肝细胞增生的IL 6为对照组 ,采用3 H TdR掺入法 ,观察HSS对大鼠肝细胞和人肝癌细胞分裂增生和细胞形态变化的影响。结果在培养早期HSS对正常大鼠肝细胞和人肝癌细胞均具有刺激增生的作用 ,随后HSS对这些细胞的增生具有明显的抑制作用 ,并伴随着细胞的死亡形态改变。结论HSS对人肝癌细胞和正常大鼠肝细胞的增生不仅有促进作用 ,而且具有较强的抑制作用 。

人胎肝细胞生长刺激物质的分离纯化及活性测定

从人胎肝组织纯化肝细胞生长刺激物质（ｈＨＳＳ），经过匀浆、热处理、乙醇沉淀、ＤＥＡＥ－ＳｅｐｈａｄｅｘＡ５０离子交换层析和ＳｅｐｈａｄｅｘＧ７５凝胶过滤，聚丙烯酰胺梯度凝胶电泳及ＩＳＣＯＣｏｎｃｅｎｔｒａｔｏｒ转移浓缩电泳等步骤，分离出具有ＨＳＳ活性的蛋白质。经ＳＤＳ－聚丙烯酰胺凝胶电泳显示５３ＫＤ与１８ＫＤ两条带。

人肝细胞刺激因子对环磷酰胺致S_(180)荷瘤小鼠肝损伤的保护作用

目的:肝细胞刺激因子(HSS)对环磷酰胺(CP)致S180荷瘤小鼠化疗性肝损伤的保护作用及可能机理。方法:采用S180荷瘤小鼠,观察HSS对CP化疗后S180荷瘤小鼠血清生化指标和肝组织匀浆氧化及抗氧化指标、肝组织病理学以及S180瘤重的影响。结果:HSS明显降低CP化疗组S180荷瘤小鼠肝组织丙二醛(MDA)含量,使肝组织谷胱甘肽(GSH)含量和超氧化物歧化酶(SOD)、过氧化氢酶(CAT)、谷胱甘肽-S-转移酶(GST)和谷胱甘肽过氧化物酶(GSH-PX)活性升高;血清谷丙转氨酶(ALT)、乳酸脱氢酶(LDH)活性,HSS治疗组与对照组、CP化疗组比较均无显著性差异;病理学检查发现CP化疗组肝组织点状及小灶性坏死,坏死区及汇管区大量炎性细胞浸润,HSS可部分逆转这些变化;HSS治疗组瘤重与CP化疗组瘤重无显著性差异。结论:CP可致S180荷瘤小鼠化疗性肝损伤,HSS具有保护作用,其抗损伤机制可能与抗氧化应激有关。

大鼠肝再生过程中肝再生刺激物及其mRNA的动态变化

本实验先制备大鼠肝再生模型，在该模型中大鼠成活率达９５％以上，肝再生情况良好，适合于进行下一步的研究。随后，通过耐热性和肝细胞特异性的检测，初步认为从该模型中所提取的活性成分即为肝再生刺激物（ＨＳＳ）。用３Ｈ胸腺嘧啶核苷测定ＨＳＳ及其ｍＲＮＡ体外翻译产物的生物活性，结果表明二者在肝再生过程中均存在动态变化，但前者在肝部分（２／３）切除后７２ｈ活性最高，后者则在２４ｈ达高峰。这一结果为后续的分子克隆工作奠定了基础。

鲨鱼肝刺激物对大鼠急性肝损伤和肝脏线粒体功能的影响

目的研究鲨鱼肝刺激物(sHSS)对硫代乙酰胺(TAA)所致大鼠急性肝损伤和肝线粒体功能的影响。方法雄性SD大鼠,体质量(200±20)g,随机分3组对照组、模型组、治疗组,每组8只。以400mg/kgTAA2次腹腔注射建立大鼠急性肝损伤模型,治疗组在注射TAA前1h腹腔注射80mg/kgsHSS,对照组注射等体积的生理盐水,24h后观察大鼠血清中丙氨酸氨基转移酶(ALT)、门冬氨酸氨基转移酶(AST)活性和肝中丙二醛(MDA)含量的变化,以及TAA和sHSS对肝线粒体呼吸功能、线粒体肿胀和膜电位的影响。结果治疗组大鼠血清中ALT、AST的水平明显低于模型组,而模型组MDA含量明显高于治疗组和正常组(P<0.05);治疗组大鼠肝脏线粒体ADP诱导的3态氧消耗、呼吸控制率(RCR)、氧化磷酸化率(OPR)明显高于TAA模型组(P<0.05);注射TAA和sHSS后,线粒体肿胀和跨膜电位没有明显的变化。结论sHSS能明显抑制TAA造成的急性肝损伤和脂质过氧化,改善因TAA而受损的线粒体呼吸功能。

鲨肝刺激物质降血糖作用机制的研究

目的 :研究鲨肝刺激物质的降血糖作用机制。方法 :采用四氧嘧啶糖尿病小鼠模型 ,观察鲨肝刺激物质对糖尿病小鼠空腹血糖、果糖胺、胰岛素、肝糖原、己糖激酶、过氧化脂质等生化指标的影响。采用离体培养原代小鼠肝细胞 ,研究鲨肝刺激物质对四氯化碳、对乙酰氨基酚所致肝细胞损伤的作用。结果 :鲨肝刺激物质显著降低糖尿病小鼠空腹血糖和果糖胺水平 ,增加血清胰岛素、肝糖原含量 ,提高己糖激酶活性 ,减轻四氯化碳、对乙酰氨基酚对原代小鼠肝细胞的损伤。结论 :鲨肝刺激物质降血糖作用机制与保护胰岛和肝细胞功能、提高己糖激酶活性。

肝细胞刺激因子对骨髓单个核细胞向肝归巢的影响

目的:探讨肝细胞刺激因子对骨髓单个核细胞(BMMNC)在小鼠体内向肝归巢的影响。方法:制备BALB/c小鼠2-乙酰氨基芴-四氯化碳肝损伤模型,供鼠分离BMMNC,体外经PKH26染色,经尾静脉途径输入肝损伤小鼠体内,实验组立即以80μg/(kg.d)剂量腹腔内注射肝细胞刺激因子,对照组注射等量5%葡萄糖溶液。移植2周后取小鼠肝,冷冻切片计荧光细胞数,苏木精-伊红(H-E)染色观察病理组织学变化。结果:实验组小鼠肝冷冻切片上平均荧光细胞数多于对照组(84vs61,P<0.05)。H-E切片上新生肝细胞较多。结论:肝细胞刺激因子对BMMNC向肝归巢有一定的促进作用。