The Relationship between 67KD Laminin Receptor Expression and Metastasis of Hepatocellular Carcinoma

The 67KD laminin receptor (LN-R ) that binds laminin (LN) is involved in the metastasis cascade. Using immunohistochemical technique, in situ hybridization and reverse transcription polymerase chain reaction(RT-PCR), we studied LN-R protein and RNA levels in 30 cases of human hepatocellular carcinoma (HCC) to further understand its role in the metastasis of HCC. In our 14 cases of HCC with metastasis, its positive rates were 71. 4 %, 57. 1%, 85.7% respectively, whereas its positive expression in 16 cases without metastasis were 31.3 %, 18. 8 %, 50. 0 % respectively. The significant difference was found between these two groups. The results suggest that the 67KD LN-R expression plays a very important role in the metastasis of HCC.

The matrix metalloproteinase stromelysin-3 cleaves laminin receptor at two distinct sites between the transmembrane domain and laminin binding sequence within the extracellular domain

The matrix metalloproteinase (MMP) stromelysin-3 (ST3) has long been implicated to play an important role in extracellular matrix (ECM) remodeling and cell fate determination during normal and pathological processes. However like other MMPs, the molecular basis of ST3 function in vivo remains unclear due to the lack of information on its physiological substrates. Furthermore, ST3 has only weak activities toward all tested ECM proteins. Using thyroid hormone-dependent Xenopus laevis metamorphosis as a model, we demonstrated previously that ST3 is important for apoptosis and tissue morphogenesis during intestinal remodeling. Here, we used yeast two-hybrid screen with mRNAs from metamorphosing tadpoles to identify potential substrate of ST3 during development. We thus isolated the 37 kd laminin receptor precursor (LR). We showed that LR binds to ST3 in vitro and can be cleaved by ST3 at two sites distinct from where other MMPs cleave. Through peptide sequencing, we determined that the two cleavage sites are in the extracellular domain between the transmembrane domain and laminin binding sequence. Furthermore, we demon strated that these cleavage sites are conserved in human LR. These results together with high levels of human LR and ST3 expression in carcinomas suggest that LR is a likely in vivo substrate of ST3 and that its cleavage by ST3 may alter cell-extracellular matrix interaction, thus, playing a role in mediating the effects of ST3 on cell fate and behavior ob- served during development and pathogenesis.

PREPARATION AND IDENTIFICATION OF MONOCLONAL ANTIBODIES AGAINST THE EXTRACELLULAR DOMAIN OF INTEGRIN a6 SUBUNIT-THE SPECIFIC LAMININ RECEPTOR

Objective: To prepare monoclonal antibody (McAb) against the Integrin α6 extracellular domain and identify its biological activities. Methods: Fusion-protein of integrin α6 extracellular domain (GST-IAGED) was expressed in E.coli. JM109 and used for immunizing BALB/C mice. The spleen cells from immunized mice were fused with SP2/0 cells and selectively cultured with HAT medium. ELISA and immunocytochemistry staining were used to select hybridomas. Results: One strain of hybridoma cells that secreted specific monoclonal antibody against integrin α6 extracellular domain was indentified. The immunoglobulin subclass of the McAb was IgG1. Conclusion: The McAb against the extracellular domain of integrin α6 was successfully prepared by using GST-IA6ED fusion protein expressed by E.Coli. And the McAb had positive reaction with human hepatocarcinoma cells-BEL-7402.

VARIATION IN MEMBRANE PROPERTIES FROM THE ACTION OF LAMININ ON MEMBRANE RECEPTORS

Biophysical studies were conducted on the action of laminin through membrane receptors of cancer cells. The results showed that variations occurred in the thermodynamic properties of membrane proteins,the mobility of hydrocarbon chains of membrane lipids, and the permeability and transportation pathways of the membrane.

THE CHARACTERISTICS OF LAMININ RECEPTOR ISOLATED FROM MURINE LUNG LEWIS CARCINOMA

Laminin receptor(LN-R, Mr=70,000) isolated from murine Lewis lung carcinoma was shown to be a single band on SDS-PAGE (Sodium Dodecyl Sulfate-Polyacrylamide gel electrophoresis) after reduction. The present study Indicates that LN-R was a kind of glycoproteins by periodic add Schiff staining. It's pI was 4. 93. LN-R preperation was associated with phospholipid and neutral glycolipid by TLC (thin layer chromatography) or HPTLC (high performance thin layer chromtography) of chloroform-methanol extracts of LN-R, respectively, but without acidic glycolipid. Binding of LN-R with its ligand, Lamlnin, depended on the presence of Ca+ + , Mg++. LN-R may bind to actin.

The interaction of laminin and its membrane receptor on mouse macrophage membrane studied by STM and FRAP

The variation of membrane surface and lateral diffusion of membrane protein was studied after the interaction of laminin with its membrane receptor in mouse macrophages. A pattern of membrane surface which showed smaller and bigger peaks was obtained by scanning tunneling microscope(STM), looking like the domains of lipid groups and proteins in the model of fluid mosaic biomembrane. Some even more higher and wider peaks projected out from the membrane surface in STM image after the interacting of laminin with membrane receptor were, probably, the complexes of laminin and membrane receptor. Furthermore, the decreased lateral diffusion coefficient value (D) was obtained by fluorescence recovery after photobleaching (FRAP) after the laminin was reacted with membrane receptor. This phenomenon provides an evidence that the complexes of laminin and its membrane receptor were located on the membrane of macrophages. So we could consider that the laminin is combined with membrane receptor leading to the variation in the properties of membrane surface.

Quantitative investigation of invasive effects of laminin-receptorantibodies on human colorectal carcinoma cell lines

Objective To investigate the relationship between expression of type Ⅳ collagenase (Ⅳ col ) andthe invasion of laminin-receptors (LNR) in human colorectal carcinoma cells. Methods: The expression ofLNR and Ⅳ col in human colorectal carcinoma(HCC) cell lines were detected quantitatively with different potential metastasis. By using human amniotic membrane(HAM) invasion model, we observed the expressionof Ⅳ col and invasion in both HCC cell lines affected by LNR monoclonal antibodies. Results: High metastaticpotential cell line Lovo expressed higher levels of LNR and Ⅳ col than HT29, a low metastatic potential HCCcell line. The number of cells adhered to HAM of Lovo were more than that of HT29. When the cells of thetwo HCC cell lines blocked by LNR antibodies, the expression of Ⅳcol were decreased, and the cells adheredto HAM expressed Ⅳ col were also decreased. Conclusion: LNR might affect the regulation of expression ofⅣ col in tumor cells by cellular signal communication, and then affect the invasion and metastasis of tumor.

稳定表达草鱼LamR鱼类细胞的建立及对基因Ⅱ型GCRV增殖的影响

通过构建草鱼LamR(Ctenopharyngodon idella LamR,CiLamR)真核表达质粒,转染GCRV非敏感细胞系鲤鱼上皮细胞(EPC)和敏感细胞系草鱼肾细胞(CIK),利用G418筛选获得稳定表达CiLamR的细胞,经Western Blot验证CiLamR稳定表达细胞系的构建。采用Ⅱ型GCRV分别接毒CiLamR稳定表达EPC和CIK,检测接毒后Ⅱ型GCRV拷贝数差异,研究草鱼37 kDa/67 kDa层粘连蛋白受体(37 kDa/67 kDa laminin receptor,LamR)对Ⅱ型GCRV增殖的影响。结果显示:经PCR扩增获得927 bp CiLamR完整开放阅读框(ORF),并成功克隆进入真核表达质粒pEYFP-Mem,获得pEYFP-Mem-CiLamR重组质粒,转染并经过G418筛选后获得约80%阳性荧光的细胞。Western Blot证实稳定表达CiLamR的EPC和CIK细胞系构建成功。以不同初始浓度接种EPC-pEYFP-Mem、EPC-pEYFP-Mem-CiLamR细胞均未检测到Ⅱ型GCRV增殖,CIK-pEYFP-Mem、CIK-pEYFP-Mem-CiLamR可检测到病毒增殖,但是增殖量无明显差异。结果表明:CiLamR蛋白对基因Ⅱ型GCRV增殖无明显影响。

^(99m)Tc-YIGSR as a Receptor Tracer in Imaging the Ehrlich Ascites Tumor-bearing Mice as Compared with ^(99m)Tc-MIBI

The validity of ^99mTc-YIGSR, a novel receptor radio-tracer, in imaging the Ehrlich ascites tumor was evaluated. YIGSR, a pentapeptide of laminin, was labeled with ^99mTc by using a bifunctional chelator S-Acetly-NH3-MAG3. The MIBI was labeled with ^99mTc by following the kit instruction. The mice of tumor group were intravenously injected 1-2 mCi of ^99mTc-YIGSR or ^99mTc-MIBI via caudal vein, immobilized and imaged under a Gamma camera. The same procedure was performed in mice of blockade group, in which the unlabeled YIGSR was previously injected to block the receptor-recognition sites, and inflammation group serving as control. The reverse-phase Sep-Pak C18 chromatogram was found to have an essentially complete conjugation between YIGSR and S-Acetly-NH3-MAG3. The conjugated YIGSR could be radio-labeled successfully with ^99mTC at room temperature and neutral pH, with a radio-labeling yield of 62%. Without the chelator S-Acetly-NH3-MAG3, the YIGSR was labeled with ^99mTc at an efficiency of 4%. The imagological study revealed obvious tumor accumulation of ^99mTc-YIGSR 15 min after the injection, and the uptake peaked after 3 h with a tumor-to-muscle ratio （T/M） of 11.36. The radio-tracer was slowly cleared up and resulted in a T/M of 3.01 at the 8th h after the injection. As for blocked group, the tumor uptake of radiotracer was significantly lower, with the highest T/M being 4.61 after 3 h and 0.89 after 8 h. The T/M was 3.72 at the 3rd h and 1.29 at the 8th h after the ^99mTc-YIGSR injection in the inflammatory group. The T/M was significantly higher in tumor group than in inflammatory group or control group （P〈0.001）. In the ^99mTc-MIBI group, the T/M was 1.40 at the 3rd h and 0.55 at the 8th h after the injection, which showed a significant difference as compared with ^99mTc-YIGSR （P〈0.001）. It is concluded that YIGSR can be successfully radiolabelled by using S-Acetly-NH3-MAG3. ^99mTc-YIGSR has many advantages in tumor imaging, such as quick and clear visualization, high sensitivity and specificity, and satisfactory target/non-target ratio （N/NT）. It promises to be tumor radio-tracer.

利用聚丙烯酰胺凝胶电泳纯化的微量蛋白制备抗血清

目的 以SDS PAGE纯化的微量蛋白制备抗人层粘连蛋白受体前体蛋白 (LRP)的血清。方法 以SDS PAGE分离纯化原核表达的人LRP与 6×组氨酸的融合蛋白 ,切下并粉碎融合蛋白所在凝胶块。将含 10 μg融合蛋白的凝胶颗粒与弗氏佐剂混匀后 ,免疫BALB/c小鼠。以Westernblot检测所获抗血清的滴度和特异性。结果 以胃癌细胞总蛋白为靶抗原时 ,Westernblot显示 ,所获抗血清仅识别 1条Mr 约 4 2 0 0 0的蛋白带 ,将抗血清做 1∶2 0 0 0稀释后 ,仍能清晰地显示其靶抗原所在位置。结论 以聚丙烯酰胺凝胶颗粒为载体 。

层粘素LN及其受体LN-R在胆管癌淋巴结转移中的作用

目的：探讨人胆管癌细胞中ＬＮ和ＬＮ—Ｒ的表达水平与胆管癌转移的关系。方法：应用 Ｓ—Ｐ免疫组化法 对５２例人胆管癌细胞中ＬＮ和 ＬＮ－Ｒ的表达水平进行研究。结果：ＬＮ及 ＬＮ－Ｒ高表达与胆管癌淋巴结转移至明显 相关， ＬＮ及 ＬＮ—Ｒ阳性肿瘤淋巴结转移率（８３％，５５％）明显高于ＬＮ—Ｒ阴性肿瘤（１５％，２０％，Ｐ＜０．０５），且ＬＮ及 ＬＮ—Ｒ 的表达与胆管癌组织学类型、分化程度亦存在明显相关（Ｐ＜０．０５）。结论：ＬＮ及ＬＮ—Ｒ的表达在胆管癌淋巴结转移中 的关系起联合作用。

胆管癌细胞层粘连蛋白受体表达下调对蛋白水解酶MMP-2、MMP-9 mRNA表达的影响

研究层粘连蛋白受体 (lamininreceptor,LNR)反义寡核苷酸硫代修饰片段 (AS OD)对人胆管癌QBC939细胞MMP 2、MMP 9基因表达的调节。应用逆转录聚合酶链反应 (RT PCR)方法分析 12 μmol/L浓度的LNRAS OD在作用 72h后对QBC939细胞MMP 2、MMP 9mRNA表达水平的影响。结果显示 ,LNRAS OD能明显抑制人胆管癌细胞表达MMP 2、MMP 9的作用 ,与正常对照相比 ,其MMP 2、MMP 9mRNA相对丰度分别下降了 33 2 %和 2 3 9% (P <0 0 5 )。研究表明 ,LNRAS OD是胆管癌细胞表达MMP 2和MMP 9基因的调节剂 ,能抑制胆管癌细胞MMP 2、MMP 9基因的表达。

肝癌细胞67kDa层粘连蛋白受体的表达

背景与目的:本实验室最近发现人肝癌细胞SMMC-7721表达的67kDa层粘连蛋白受体(67kDaLamininreceptor,67LR)与层粘连蛋白的结合能力明显高于正常肝细胞L-02表达的67LR,而67LR在肝癌细胞和正常肝细胞中的表达水平尚不清楚。本研究旨在探讨67LR在肝癌细胞中的表达,及其与层粘连蛋白结合能力的关系。方法:以人肝癌细胞SMMC-7721、HepG2和正常肝细胞L-02为材料,采用131I标记的层粘连蛋白测定其与细胞的结合能力;采用流式细胞术和RT-PCR分析67LR蛋白和mRNA的表达水平。结果:(1)相同条件下SMMC-7721、HepG2细胞与层粘连蛋白特异结合量分别为(17.54±0.49)ng/105cell、(11.18±0.53)ng/105cell,而L-02细胞的特异结合量为(8.36±0.48)ng/105cell,表明肝癌细胞与层粘连蛋白的结合能力明显高于正常肝细胞(P<0.01);(2)流式细胞术分析,SMMC-7721细胞的67LR阳性表达率为34.7%,L-02细胞的67LR阳性表达率为55.3%,而HepG2细胞则几乎不表达67LR;(3)RT-PCR产物进行半定量分析发现,两株肝癌细胞的67LRmRNA表达水平明显高于L-02细胞。结论:肝癌细胞与层粘连蛋白的结合能力明显高于正常肝细胞L-02,而细胞膜表面的67LR水平却低于L-02细胞,提示SMMC-7721细胞67LR的亲和力可能高于L-02细胞,而且还涉及其它层粘连蛋白受体。

层粘连蛋白受体单克隆抗体对人肺癌细胞形态、粘着及铺展的影响

应用体外细胞培养，观察了层粘连蛋白受体单克隆抗体（ＭｃＢ＿１）加入培养液或预处理人肺巨细胞癌（ＰＧ）和肺腺癌（ＰＡａ）后某些生物学行为的改变。在体外ＭｃＢ＿１预孵育可抑制ＰＧ和ＰＡａ在层粘连蛋白基质上的粘着和铺展。培养液中加入ＭｃＢ＿１经扫描电镜观察，ＭｃＢ＿１明显改变该两种细胞的表面形态。说明层粘连蛋白受体在肿瘤浸润和转移中可能起重要作用。层粘连蛋白受体单克隆抗体在阻断肿瘤转移的发生上可能具有应用价值。

层粘连蛋白及其受体在妊娠滋养细胞肿瘤中的表达及意义

目的 了解葡萄胎、侵蚀性葡萄胎和绒毛膜癌组织中层粘连蛋白(L N )及其受体(L N - R)的表达,并探讨L N、L N - R与妊娠滋养细胞肿瘤(GTT)侵袭和转移的关系。方法 以4 4例恶性GTT为研究组,2 4例葡萄胎为对照组,采用免疫组化方法对两组患者首次清宫标本组织进行L N,L N- R检测。结果 L N在绒毛膜癌组织中临床分期越晚,表达率越高,其表达与绒毛膜癌细胞的浸润转移以及恶性程度有一定关系。结论 化疗对L N、L N- R在妊娠滋养细胞肿瘤中的表达有一定的影响,推测L N和L N- R在妊娠滋养细胞肿瘤抗侵袭和转移治疗方面具有潜在的应用价值。

67kD层粘连蛋白受体的克隆、表达及其对肝癌细胞侵袭能力的影响

探讨细胞膜表面 6 7kD层粘连蛋白受体 (6 7kDlamininreceptor ,6 7LR)在肝癌细胞侵袭转移中的作用 ,从肝癌细胞中提取RNA ,通过RT PCR扩增 6 7LR的前体——— 37kD层粘连蛋白受体前体(37kDlamininreceptorprecursor,37LRP)基因并定向克隆到真核表达载体pcDNA3.1 myc His(- )A ,采用脂质体将重组质粒转染到HepG2肝癌细胞中 ,通过G4 1 8筛选和RT PCR、流式细胞术鉴定 ,获得了细胞膜表面 6 7LR高表达 (阳性率为 6 9.2 % )和低表达 (阳性率为 1 1 .7% )的细胞克隆 ,采用体外细胞侵袭实验测定不同细胞的侵袭能力 ,发现膜表面 6 7LR高表达的细胞侵袭能力明显高于低表达及不表达细胞 ,说明 6

MMP-9和层粘连蛋白受体在乳腺癌组织中的表达及其与转移和预后的关系

背景与目的:以往对乳腺癌细胞外基质与肿瘤转移及患者预后之间关系的研究尚少,且结论不一。本研究探讨乳腺癌组织中基质金属蛋白酶-9(matrixmetalloproteinase-9,MMP-9)及层粘连蛋白受体(lamininreceptor,LM-R)表达与肿瘤转移及患者预后的关系。方法:应用免疫组化方法检测80例乳腺癌组织及10例乳腺增生病组织中MMP-9、LM-R的表达,并用计算机图像分析系统测定表达的吸光度值。采用t检验、方差分析及相关分析方法分析它们与肿瘤转移和患者预后的关系。结果:乳腺癌组织中MMP-9表达显著高于乳腺增生病(t=8.87,P<0.05);在乳腺增生病组织中,LM-R表达于基底膜及部分腺泡和导管的腔缘,在乳腺癌组织中表达于细胞质及胞膜;17例癌间质血管基底膜有LM-R表达的癌组织中,LM-R表达高于血管基底膜无LM-R表达组(t=2.02,P<0.05);LM-R表达与组织学分级有关,分化低者,表达水平高(F=3.27,P<0.05);MMP-9及LM-R表达均与淋巴结转移有关,它们在有3个以上淋巴结转移组的表达低于3个以下及无转移组(tMMP-9=3.42,tLM-R=4.31,P<0.05),原发灶与转移灶的表达呈正相关(rMMP-9=0.654,rLM-R=0.755,P<0.001);MMP-9与孕激素受体负相关性(r=-0.363,P<0.05);MMP-9与LM-R之间呈正相关(r=0.503,P<0.01)。

胃腺癌组织层粘连蛋白受体表达的意义

目的:探讨LN-R在判断胃腺癌浸润转移及预后中的作用方法:应用免疫组织化学S-P法检测76例胃腺癌组织和10例正常胃组织中LN—R的表达水平,比较LN—R的不同表达率与生存率的关系. 结果:LN—R在胃腺癌组织中阳性表达率为51.3%,较正常组织(10.0%)显著增高(P<0.05),与分化程度、Borrmann分型、浸润深度、肿块大小、淋巴结转移程度比较关系显著(X2=10.606、9.979、6.838、7.611、12.509,P<0.05),LN-R阳性表达者的生存时间较阴性者短(X2=9.980,P<0.05).

绝经后女性盆底脏器脱垂患者阴道前壁组织中层粘连蛋白、胶原蛋白及雌激素受体的表达

目的研究绝经后女性盆底脏器脱垂患者阴道前壁组织中层粘连蛋白(LN)、胶原蛋白及雌激素受体(ER)的表达。方法选择2016年1月至2018年12月于上海市嘉定区妇幼保健院因绝经后盆底脏器脱垂行阴式全子宫切除术+阴道壁修补术的40例患者作为观察组;另选择同期因其他子宫良性病变行阴式子宫全切术的40例患者作为对照组。术前采用酶联免疫吸附试验检测2组患者血清LN水平;术中取2组患者阴道前壁组织,采用荧光定量聚合酶链反应法检测LN mRNA表达,采用免疫组织化学法检测LN、胶原蛋白Ⅰ、胶原蛋白Ⅲ及ER表达。结果术前,观察组与对照组患者血清LN水平比较差异无统计学意义(P>0.05)。观察组患者阴道前壁组织中LN mRNA的相对表达量显著低于对照组(P<0.05)。观察组和对照组患者阴道前壁组织中LN阳性表达率分别为12.5%(5/40)、27.5%(11/40),观察组患者阴道前壁组织中LN阳性表达率显著低于对照组(χ2=45.262,P<0.01)。观察组患者阴道前壁组织中胶原蛋白Ⅰ、胶原蛋白Ⅲ及ER表达评分均显著低于对照组(P<0.05)。结论LN、胶原蛋白Ⅰ、胶原蛋白Ⅲ及ER在绝经后女性盆底脏器脱垂患者阴道前壁组织中的表达降低,推测绝经后女性盆底脏器脱垂与以上因素有关。

米非司酮药流后子宫出血机理探讨

目的: 探讨米非司酮药流后子宫出血的机理。 方法:采集正常早孕人工流产、药物流产完全与不完全蜕膜组织各20例,应用免疫组化法表达组织中的PR、Fas、LN、FN,应用图象分析仪及半定量方法对表达结果进行观察(P<0.01)。结果: 药流不全组PR、LN的表达均明显高于药流完全组(P<0.05和P<0.01),而Fas表达则明显低于药流完全组(P<0.01)。结论: 药流不全组PR的高表达导致蜕膜组织凋亡障碍,并持续分泌LN致使蜕膜组织粘连不脱落,子宫持续出血,而PR高表达的原因有可能归于使用者的个体差异。