Expression and Immune Effect of Toll-Like Receptor 4 in Human Trophoblast Cells

This study investigated the expression and immune effect of TLR4 in human trophoblast cells. The expression level of TLR4 mRNA in normal and LPS-stimulated human term trophoblast cells （1 mg/L LPS, 12 h） was detected by RT-PCR. In LPS-stimulated human term trophoblast cells of TLR4-blocked group and non-TLR4-blocked group, and normal term trophoblast cells of blank control group, apoptosis rate was measured by flow cytometry （FCM）, and the level of TNF-α determined by using enzyme linked immunosorbent assay （ELISA） respectively. RT-PCR results showed that the expression level of TLR4 mRNA in LPS-stimulated human trophoblast cells was significantly higher than that in normal cells （P〈0.01）. FCM revealed that there was significant difference in apoptosis rate of LPS-stimulated human term trophoblast cells between TLR4-blocked group and non-TLR4-blocked group （P〈0.05）, or between TLR4 antibody-blocked group and blank control group. ELISA indicated that the level of TNF-α in LPS-stimulated human trophoblast cells also had statistical differences between TLR4 antibody-blocked group and non-TLR4 antibody-blocked group （P〈0.05）. Our results suggest that TLR4 plays an important role in the immunological mechanism of apoptosis and secretion of TNF-α of human term trophoblast cells stimulated by LPS.

Bone morphogenetic protein-4 affects both trophoblast and non-trophoblast lineage-associated gene expression in human embryonic stem cells

Human embryonic stem cells (hESC) can be induced to differentiate to trophoblast by bone morphogenetic proteins (BMPs) and by aggregation to form embryoid bodies (EB), but there are many differences and controversies regarding the nature of the differentiated cells. Our goals herein were to determine if BG02 cells form trophoblast-like cells (a) in the presence of BMP4-plus-basic fibroblast growth factor (FGF-2) and (b) upon EB formation, and (c) whether the BMP4 antagonist noggin elicits direct effects on gene expression and hormone production in the cells. Transcriptome profiling of hESC incubated with BMP4/FGF-2 showed a down-regulation of pluripotency-associated genes, an up-regulation of trophoblast-associated genes, and either a down-regulation or no change in gene expression for many markers of the three embryonic germ layers. Yet, there was up-regulation of several genes associated with mesoderm, ectoderm, and endoderm, strongly suggesting that differentiation to trophoblast-like cells under the conditions used does not yield a homogeneous cell type. Several genes, heretofore unreported, were identified that are altered in hESC in response to BMP4-mediated differentiation. The production of human chorionic gonadotropin (hCG), progesterone, and estradiol in the differentiated cells confirmed that trophoblast-like cells were obtained. Gene expression by EB was characterized by an up-regulation of a number of genes associated with trophoblast, ectoderm, endoderm, and mesoderm, and the production of hCG and progesterone confirmed that trophoblast-like cells were formed. These results suggest that, in the presence of FGF-2, BG02 cells respond to BMP4 to yield trophoblast-like cells, which are also obtained upon EB formation. Thus, BMP4-mediated differentiation of hESC represents a viable cell system for studying early developmental events post-implantation;however, up-regulation of non-trophoblast genes suggests a somewhat diverse response to BMP4/FGF-2. Noggin altered the transcription of a limited number of genes but, not surprisingly, did not lead to secretion of hormones.

Human papillomavirus 16 E6 is associated with the nuclear matrix of esophageal carcinoma cells

AIM: To explore the etiologic role of HPV infection in esophageal carcinoma, and the association of HPV-16 E6with the nuclear metrix of carcinoma cells.METHODS: Two esophageal carcinoma cell lines, EC/CUHK1 and EC/CUHK2, were tested for HPV-16 E6subgenetic fragment by polymerase chain reaction amplification of virus DNA associated nuclear matrix. RT-PCR and immunocytochemistry were also used to visualizethe expression of E6 subgene in the cells.RESULTS: The HPV-16 E6 subgenetic fragment wes found to be present in nuclear metrix-associeted DNA, E6oncoprotein localized in the nucleus where it is tightly associated with nuclear matrix after sequential extraction in EC/CUHK2 cells. It was not detected, however, in EC/CUHK1 cells.CONCLUSION: The interaction between HPV-16 E6 and nuclear matrix may contribute to the virus induced carcinogenesis in esophageal carcinoma.

How and Why Do Gestational Trophoblastic Neoplasms Overproduce Human Chorionic Gonadotropin?

From the published data, the present mini-review attempts to answer two fundamental questions about the gestational trophoblastic neoplasms. In addition, it extrapolates the findings to other cancers that produce small amounts of hCG and how a novel therapies could be developed.

Reduction of tumorigenicity of SMMC-7721 hepatoma cells by vascular endothelial growth factor antisense gene therapy

AIM: To test the hypothesis to block VEGF expression of SMMC-7721 hepatoma cells may inhibit tumor growth using the rat hepatoma model. METHODS: Amplify the 200 VEGF cDNA fragment and insert it into human U6 gene cassette in the reverse orientation transcribing small antisense RNA which could specifically interact with VEGF165, and VEGF121 mRNA. Construct the retroviral vector containing this antisense VEGF U6 cassette and package the replication-deficient recombinant retrovirus. SMMC-7721 cells were transduced with these virus and positive clones were selected with G418. PCR and Southern blot analysis were performed to determine if U6 cassette integrated into the genomic DNA of positive clone. Transfected tumor cells were evaluated for RNA expression by ribonuclease protection assays. The VEGF protein in the supernatant of parental tumor cells and genetically modified tumor cells was determined with ELISA. In vitro and in vivo growth properties of antisense VEGF cell clone in nude mice were analyzed. RESULTS: Restriction enzyme digestion and PCR sequencing verified that the antisense VEGF RNA retroviral vector was successfully constructed.After G418 selection, resistant SMMC-7721 cell clone was picked up. PCR and Southern blot analysis suggested that U6 cassette was integrated into the cell genomic DNA. Stable SMMC-7721 cell clone transduced with U6 antisense RNA cassette could express 200 bp small antisense VEGF RNA and secrete reduced levels of VEGF in culture condition. Production of VEGF by antisense transgene-expressing cells was 65+/-10 ng/L per 10(6) cells, 42045 ng/L per 10(6) cells in sense group and 485+/-30 ng/L per 10(6) cells in the negative control group, (P【 0.05). The antisense-VEGF cell clone appeared phenotypically indistinguishable from SMMC-7721 cells and SMMC-7721 cells transfected sense VEGF. The growth rate of the antisense-VEGF cell clone was the same as the control cells. When S.C. was implanted into nude mice, growth of antisense-VEGF cell lines was greatly inhibited compared with control cells. CONCLUSION: Expression of antisense VEGF RNA in SMMC-7721 cells could decrease the tumorigenicity, and antisense-VEGF gene therapy may be an adjuvant treatment for hepatoma.

Dynamic change of Adamalysin 19 (ADAM19) in human placentas and its effects on cell invasion and adhesion in human trophoblastic cells

Human ADAM19 is a recently identified member of the ADAM family.It is highly expressed in human placentas,but its dynamic change and function at the human feto-maternal interface during placentation remain to be elucidated.In this present study,the spatial and temporal expression and cellular localization of ADAM19 in normal human placentas were first demonstrated,and the effects of ADAM19 on trophoblast cell adhesion and invasion were further investigated by using a human choriocarcinoma cell line(JEG-3) as an in vitro model.The data demonstrated that ADAM19 was widely distributed in villous cytotrophoblast cells,syncytiotrophoblast cells,column trophoblasts,and villous capillary endothelial cells during early pregnancy.The mRNA and protein level of ADAM19 in placentas was high at gestational weeks 8-9,but diminished significantly at mid-and term pregnancy.In JEG-3 cells,the overexpression of ADAM19 led to diminished cell invasion,as well as increases in cell adhesiveness and the expression of E-cadherin,with no changes in β-catenin expression observed.These data indicate that ADAM19 may participate in the coordinated regulation of human trophoblast cell behaviors during the process of placentation.

The prognostic molecular markers in hepatocellular carcinoma

The prognosis of hepatocellular carcinoma (HCC) still remains dismal, although many advances in its clinical study have been made. It is important for tumor control to identify the factors that predispose patients to death. With new discoveries in cancer biology, the pathological and biological prognostic factors of HCC have been studied quite extensively. Analyzing molecular markers (biomarkers) with prognostic significance is a complementary method. A large number of molecular factors have been shown to associate with the invasiveness of HCC, and have potential prognostic significance. One important aspect is the analysis of molecular markers for the cellular malignancy phenotype. These include alterations in DNA ploidy, cellular proliferation markers (PCNA, Ki-67, Mcm2, MIB1, MIA, and CSE1L/CAS protein), nuclear morphology, the p53 gene and its related molecule MD M2, other cell cycle regulators (cyclin A, cyclin D, cyclin E, cdc2, p27, p73), oncogenes and their receptors (such as ras, c-myc, c-fms, HGF, c-met, and erb-B receptor family members), apoptosis related factors (Fas and FasL), as well as telomerase activity. Another important aspect is the analysis of molecular markers involved in the process of cancer invasion and metastasis. Adhesion molecules (E-cadherin, catenins, serum intercellular adhesion molecule-1, CD44 variants), proteinases involved in the degradation of extracellular matrix (MMP-2, MMP-9, uPA, uPAR, PAI), as well as other molecules have been regarded as biomarkers for the malignant phenotype of HCC, and are related to prognosis and therapeutic outcomes. Tumor angiogenesis is critical to both the growth and metastasis of cancers including HCC, and has drawn much attention in recent years. Many angiogenesis-related markers, such as vascular endothelial growth factor (VEGF), basic fibroblast growth factor (bFGF), platelet-derived endothelial cell growth factor (PD-ECGF), thrombospondin (TSP), angiogenin, pleiotrophin, and endostatin (ES) levels, as well as intratumor microvessel density (MVD) have been evaluated and found to be of prognostic significance. Body fluid (particularly blood and urinary) testing for biomarkers is easily accessible and useful in clinical patients. The prognostic significance of circulating DNA in plasma or serum, and its genetic alterations in HCC are other important trends. More attention should be paid to these two areas in future. As the progress of the human genome project advances, so does a clearer understanding of tumor biology, and more and more new prognostic markers with high sensitivity and specificity will be found and used in clinical assays. However, the combination of some items, i.e., the pathological features and some biomarkers mentioned above, seems to be more practical for now.

Expression of vascular endothelial growth factor and its role in oncogenesis of human gastric carcinoma

AIM: To establish the role of vascular endothelial growth factor (VEGF) in the oncogenesis of human gastric carcinoma more directly. METHODS: The expression of VEGF and its receptor kinase-domain insert containing receptor (KDR) in human gastric cancer tissue were observed by immunohistochemical staining. VEGF levels were manipulated in human gastric cancer cell using eukaryotic expression constructs designed to express the complete VEGF(165) complimentary DNA in either the sense or antisense orientation. The biological changes of the cells were observed in which VEGF was up-regulated or down-regulated. RESULTS: VEGF-positive rate was 50%, and VEGF was mainly localized in the cytoplasm and membrane of the tumor cells, while KDR was mainly located in the membrane of vascular endothelial cells in gastric cancer tissues and peri-cancerous tissue. In 2 cases of 50 specimens, the gastric cancer cells expressed KDR, localized in both the cytoplasm and membrane. Introduction of VEGF(165) antisense into human gastric cancer cells (SGC-7901, immunofluorescence intensity, 31.6%)) resulted in a significant reduction in VEGF-specific messenger RNA and total and cell surface VEGF protein (immunofluorescence intensity, 8.9%) (P【0.05). Conversely, stable integration of VEGF(165) in the sense orientation resulted in an increase in cellular and cell surface VEGF (immunofluorescence intensity, 75.4%) (P【0.05). Lowered VEGF levels were associated with a marked decrease in the growth of nude mouse xenografted tumor (at 33 days postimplantation, tumor volume: 345.40 +/- 136.31 mm3)(P【0.05 vs control SGC-7901 group: 1534.40 +/- 362.88 mm3), whereas up-regulation of VEGF resulted in increased xenografted tumor size (at 33 days postimplantation, tumor volume: 2350.50 +/- 637.70 mm3) (P【0.05 vs control SGC-7901 group). CONCLUSION: This study provides direct evidence that VEGF plays an important role in the oncogenesis of human gastric cancer.

Regulation of activin A in cell proliferation and hormone secretion by human normal trophoblast cells

Regulation of activin A in cell proliferation as well as hCG and progesterone secretion was investigated using primary cultured cytotrophoblast cells and normal placenta origin cytotrophoblast cell line-NPC cells in serum-free system. It was shown that activin A promoted hCG and progesterone secretion in primary cultured cytotrophoblast cells as well as progesterone secretion in NPC cells, while it had no effect on cell proliferation and hCG secretion in NPC cells. lmportant evidence is provided for the autocrine regulatory mechanism of activin A on hormone secretion in placental trophoblast cells at early pregnancy.

Effect of Leptin on Cytotrophoblast Proliferation and Invasion

The effects of leptin on cytotrophoblast proliferation and invasion activity were investigated. Immunohistochemistry was used to determine the placental expression of leptin in first-trimester pregnancy. By using RT-PCR and quantitative real-time PCR, the expression of leptin in cytotrophoblast and the effect of leptin on cytotrophoblast secretion were detected. The potential of cell proliferation, invasiveness and migration was assessed by MTT, Transwell invasion assay and migration assay respectively when the cytotrophoblast was cultured with different concentrations of leptin. The results showed that： （1） Leptin was distributed diffusely around cell membrane, in cytoplasma, and on nuclear mem- brane of cytotrophoblast; （2） Leptin mRNA was expressed in cytotrophoblast. Ten ng/mL leptin could promote the secretion of cytotrophoblast significantly （P〈0.01）; （3） After culture with different concentrations of leptin for 24 h or longer, the proliferation of cytotrophoblast was inhibited, while in 24 h leptin could promote cytotrophoblast invasion and migration. Leptin at a concentration of 500 ng/mL could promote cytotrophoblast invasiveness and migration significantly as compared with controls （P〈0.05）. It was suggested that leptin could inhibit cytotrophoblast proliferation, and promote cytotro- phoblast invasion and migration activity.

黄芪甲苷对高糖诱导人绒毛膜滋养层细胞(HTR-8/SVneo)焦亡及侵袭迁移的影响

【目的】探讨黄芪甲苷对高糖诱导的人绒毛膜滋养层细胞(HTR-8/SVneo)焦亡及侵袭迁移的影响。【方法】将HTR-8/SVneo细胞分为4组:对照组(未处理)、高糖组(高糖刺激)及黄芪甲苷50、100μmol/L组(高糖刺激+黄芪甲苷)。采用细胞计数试剂盒8(CCK-8)法检测细胞活力,分别采用Transwell实验和划痕实验测定细胞侵袭、迁移能力,Hoechst 33342/碘化丙啶(PI)双荧光染色评估细胞焦亡情况,蛋白免疫印迹(Western Blot)法检测细胞NOD样受体热蛋白结构域相关蛋白3(NLRP3)、胱天蛋白酶剪切体(cleaved-Caspase-1)、消皮素D-N端(GSDMD-NT)、白细胞介素18(IL-18)蛋白表达水平。【结果】与对照组比较,高糖组HTR-8/SVneo细胞活力显著降低,细胞迁移率显著降低,侵袭细胞数显著减少,PI阳性细胞比例显著增加,NLRP3、cleaved-Caspase-1、GSDMD-NT、IL-18蛋白表达水平显著升高(P<0.05或P<0.01);与高糖组比较,黄芪甲苷处理组细胞活力显著升高,细胞迁移率显著增加,侵袭细胞数显著增加,PI阳性细胞比例显著下降,NLRP3、cleaved-Caspase-1、GSDMD-NT、IL-18蛋白表达水平显著下降(P<0.05或P<0.01)。【结论】黄芪甲苷可抑制高糖诱导的HTR-8/SVneo细胞焦亡,改善细胞侵袭及迁移能力。

采用miR-148a低表达人绒毛膜滋养细胞构建的子痫前期模型细胞活力、焦亡、炎性和氧化应激反应观察

目的观察采用微小RNA-148a(miR-148a)低表达人绒毛膜滋养细胞系HTR-8/SVneo构建的子痫前期(Preeclampsia,PE)模型细胞的细胞活力、焦亡、炎症和氧化应激反应。方法取对数生长期人绒毛膜滋养细胞系HTR-8/SVneo,分为甲、乙、丙、丁组:甲组细胞用抑制miR-148a表达的miR-148a inhibitor转染24 h,加入100 ng/L的LPS培养24 h(建立PE模型);乙组细胞用空白对照NC-inhibitor转染24 h,加入100 ng/L的LPS培养24 h;丙组加入100 ng/L的LPS培养24 h;丁组不做任何处理。培养48 h时,采用qRT-PCR法检测各组细胞miR-148a,采用CCK8法检测各组细胞活力,采用TUNEL法测算各组细胞焦亡率,采用Western Blotting法检测各组细胞焦亡相关蛋白Caspase-1、GSDMD,采用ELISA法检测各组上清液炎症因子[肿瘤坏死因子α(TNF-α)、白细胞介素1β(IL-1β)、IL-6]及氧化应激指标[谷胱甘肽过氧化物酶(GSH)、超氧化物歧化酶(SOD)、丙二醛(MDA)]。结果与丁组相比,丙组细胞miR-148a相对表达量高,培养24、48、72 h时OD值低,细胞焦亡率高,细胞Caspase-1、GSDMD蛋白相对表达量高(P均<0.05);与乙组相比,甲组细胞miR-148a相对表达量低,培养24、48、72 h时OD值高,细胞焦亡率低,细胞Caspase-1、GSDMD和NLRP3蛋白相对表达量低(P均<0.05)。与丁组相比,丙组细胞上清液TNF-α、IL-1β及IL-6水平高,细胞GSH和SOD表达降低、MDA表达升高(P均<0.05);与乙组相比,甲组细胞上清液TNF-α、IL-1β及IL-6水平低,细胞GSH和SOD表达升高、MDA表达降低(P均<0.05)。结论miR-148a低表达HTR-8/SVneo细胞构建的PE模型细胞活力高,细胞焦亡程度、炎性反应及氧化应激反应低。miR-148a可能是PE的治疗靶点之一。

胃癌组织中SDF-1、HER2及Slug表达与患者临床病理特征的相关性

目的分析基质细胞衍生因子1(SDF-1)、人表皮生长因子受体2(HER2)、锌指转录因子(Slug)在胃癌组织内的表达及与患者临床病理特征间的关系。方法选取73例胃癌患者,采集其癌组织与癌旁正常组织,以免疫组织化学法检测对比两者SDF-1、HER2及Slug的表达差异;另收集患者的年龄等资料,统计分析SDF-1、HER2及Slug表达与胃癌患者各项临床病理特征间的联系。结果癌组织的SDF-1、HER2、Slug阳性表达率高于癌旁正常组织,差异有统计学意义(P<0.05)。SDF-1、HER2、Slug阳性表达与胃癌患者的年龄、性别无关(P>0.05),与患者的临床分期、淋巴结转移、分化程度有关(P<0.05)。结论SDF-1、HER2、Slug在胃癌组织内呈异常高表达,且其参与胃癌的侵袭、发展过程。

硒介导PI3K/Akt/mTOR信号通路对子痫前期滋养细胞自噬的调控作用及机制

目的探讨硒通过PI3K/Akt/mTOR信号通路对子痫前期(PE)人绒毛膜滋养细胞(HTR-8-Svneo)自噬及增殖迁移的影响及其机制。方法体外培养HTR-8-Svneo,随机分为正常对照组、乏氧组以及乏氧加硒组;对照组HTR-8-Svneo细胞置于37℃CO_(2)培养箱,乏氧组HTR-8-Svneo细胞置于37℃乏氧培养箱,乏氧加硒组HTR-8-Svneo细胞置于37℃乏氧加硒(硒浓度为10μmol/L)培养箱,三组均培养24 h。采用CCK-8试剂盒测量HTR-8-Svneo细胞活性,细胞划痕试验检测HTR-8-Svneo细胞增殖迁移能力,Western blotting法检测HTR-8-Svneo细胞PI3K/Akt/mTOR信号通路蛋白(p-PI3K、p-AKT、p-mTOR)以及自噬相关蛋白(LC3、Beclin-1、p62)表达,免疫荧光观察HTR-8-Svneo细胞LC3表达量。结果对照组、乏氧组、乏氧加硒组细胞活力OD值分别为1.5±0.21、1.04±0.05、1.48±0.27;乏氧组细胞活力较对照组降低、乏氧加硒组细胞活力较乏氧组增强(P均<0.05)。对照组、乏氧组、乏氧加硒组细胞划痕愈合率分别为17.25%、6.08%、18.13%;乏氧组细胞较对照组划痕愈合率降低、乏氧加硒组较乏氧组细胞划痕愈合率升高(P均<0.05)。乏氧组与对照组、乏氧加硒组与乏氧组比较,HTR-8-Svneo细胞通路蛋白以及自噬相关蛋白表达差异有统计学意义(P均<0.05)。对照组、乏氧组、乏氧加硒组HTR-8-Svneo细胞荧光表达量分别为73.26±4.18、134.83±3.03、74.7±12.37;乏氧组细胞荧光表达量较对照组升高,乏氧加硒组细胞荧光表达量较乏氧组降低,差异均有统计学意义(P均<0.05)。结论HTR-8-Svneo细胞加硒培养可提高细胞活力和增殖迁移能力,其机制可能与硒通过PI3K/AKT/mTOR通路调控PE滋养细胞自噬相关。

SHP-2对人绒毛膜滋养层细胞增殖、侵袭、迁移和PI3K/AKT信号通路蛋白表达的影响

目的探讨Src同源物2磷酸酶2(SHP-2)对人绒毛膜滋养层细胞HTR-8/SVneo增殖、侵袭、迁移和PI3K/AKT信号通路蛋白表达的影响。方法用定量实时聚合酶链反应(qRT-PCR)检测SHP-2在子痫前期(PE)组胎盘组织中的表达水平。采用细胞计数试剂盒-8(CCK-8)、克隆形成实验、划痕闭合和Transwell分析检测敲低或过表达SHP-2对人绒毛膜滋养细胞(HTR-8/SVneo)增殖、集落形成、迁移和侵袭能力的影响。Western blot检测侵袭相关蛋白的表达和磷脂酰肌醇3激酶(PI3K)、蛋白激酶B(AKT)的磷酸化水平。结果HP-2在PE组胚胎组织中低表达。敲低SHP-2显著抑制HTR-8/SVneo细胞的增殖、集落形成、侵袭和迁移,此外,基质金属蛋白酶-2(MMP-2)、N-钙黏蛋白(N-cadherin)和波形蛋白(Vimentin)的表达显著下调,E-钙黏蛋白(E-cadherin)表达显著上调,PI3K和AKT的磷酸化水平显著降低,然而,过表达SHP-2具有相反的效果。结论SHP-2在PE胎盘组织中低表达,SHP-2过表达可促进滋养层细胞的增殖、侵袭和迁移能力,提示SHP-2可能是临床治疗PE的潜在靶点。

抗体偶联药物在非小细胞肺癌中的研究进展

肺癌是全球发病率第一位、病死率第二位的恶性肿瘤。非小细胞肺癌(non-small cell lung cancer,NSCLC)是最主要的肺癌病理分型。目前晚期NSCLC的一线标准治疗方案为免疫治疗、靶向治疗,虽然延长了患者的生存期,但获得性耐药仍是不可避免的。抗体偶联药物(antibody-drug conjugates,ADCs)是一类经由连接子将细胞毒性载荷与特异性单克隆抗体偶联制成的新型抗肿瘤药物,与化疗药物相比,ADCs具有精准识别、局部释放、患者耐受性高等优点,近年在NSCLC治疗方面显示出良好的临床获益。本文针对ADCs的作用机制、在晚期NSCLC中的临床研究进展以及存在的问题和挑战等方面进行概述。

miR-30c-5p对人绒毛滋养层细胞线粒体自噬、间充质转化及PEG10水平影响

目的探讨miR-30c-5p对人绒毛滋养层细胞线粒体自噬、间充质转化及PEG10水平影响。方法人绒毛滋养层细胞HTR-8/SVneo分为空白组(HTR-8/SVneo细胞正常培养)、低氧组(HTR-8/SVneo细胞低氧培养)、miR-30c-5p mimics组(HTR-8/SVneo细胞低氧培养转染miR-30c-5p mimics)、NC-mimics组(HTR-8/SVneo细胞低氧培养转染NC-mimics)、miR-30c-5p inhibitor组(HTR-8/SVneo细胞低氧培养转染miR-30c-5p inhibitor)、NC-inhibitor组(HTR-8/SVneo细胞低氧培养转染NC-inhibitor)。qRT-PCR检测各组细胞miR-30c-5p表达;Transwell小室检测细胞侵袭数目;划痕试剂盒检测细胞划痕愈合率;相关试剂盒检测ROS水平;免疫印记检测PEG10、Parkin、PINK1蛋白水平。结果空白组、低氧组、miR-30c-5p mimics组、NC-mimics组、miR-30c-5p inhibitor组及NC-inhibitor组的miR-30c-5p表达分别为1.00±0.00、1.00±0.00、1.61±0.15、1.03±0.13、0.75±0.08及0.96±0.10,差异有统计学意义(F=45.750,P<0.05);与空白组相比,低氧组HTR-8/SVneo细胞侵袭数目、划痕愈合率、PEG10、Parkin、PINK1降低,ROS升高,差异均有统计学意义(P<0.05);低氧组与NC-mimics组、NC-inhibitor组比较上述指标,差异均无统计学意义(P>0.05);与低氧组相比,miR-30c-5p mimics组细胞侵袭数目、划痕愈合率、PEG10、Parkin、PINK1降低,ROS升高,差异均有统计学意义(P<0.05),miR-30c-5p inhibitor组细胞侵袭数目、划痕愈合率、PEG10、Parkin、PINK1升高,ROS降低,差异均有统计学意义(P<0.05)。结论抑制miR-30c-5p可加快低氧状态下的人绒毛滋养层细胞侵袭及迁移,并通过促进线粒体自噬降低ROS表达,机制与抑制PEG10水平相关。

滋养层细胞表面抗原2在肝细胞腺瘤和肝细胞肝癌的表达及意义

目的:探讨滋养层细胞表面抗原2(Trop2)在肝细胞腺瘤(HCA)和肝细胞肝癌(HCC)的表达及意义。方法:收集2018—2021年南方医科大学附属小榄医院病理科收治的59例HCC患者、4例HCA患者的手术切除标本。采用免疫组化方法检测HCA和HCC中Trop2的表达,并计数微血管密度(MVD)和胆管反应(DR)。结果:Trop2标记间质DR与肝细胞腺瘤相比,肝细胞肝癌的间质DR减少或缺失,CD34标记的MVD降低。Pearson相关分析结果显示,Trop2小DR与CD34 MVD呈正相关(r=0.488,P<0.001)。结论:Trop2在促进肿瘤的发生发展及转移中有一定的作用。

乳腺癌组织HER-2、Ki67表达水平及其与病理参数的相关性

目的:分析乳腺癌组织人表皮生长因子受体-2(HER-2)、细胞增殖核抗原(Ki67)表达水平及其与病理参数的相关性。方法:回顾性分析2021年9月至2023年4月该院收治的70例乳腺癌患者的临床资料,采用免疫组织化学染色法检测患者癌组织HER-2、Ki67表达水平,比较不同病理参数乳腺癌患者癌组织HER-2、Ki67表达水平,并分析其与病理参数的相关性。结果:70例乳腺癌患者中,癌组织HER-2阳性54例,阳性率为77.14%(54/70);Ki67阳性47例,阳性率为67.14%(47/70);不同年龄、病理类型乳腺癌患者癌组织HER-2、Ki67阳性率比较,差异均无统计学意义(P>0.05);不同淋巴结转移、临床分期、肿瘤直径乳腺癌患者癌组织HER-2、Ki67阳性率比较,差异均有统计学意义(P<0.05);Pearson相关性分析结果显示,乳腺癌组织HER-2、Ki67表达水平与淋巴结转移、临床分期、肿瘤直径均呈正相关(r>0,P<0.05)。结论:乳腺癌组织HER-2、Ki67表达水平与淋巴结转移、临床分期、肿瘤直径均呈正相关。

人早孕绒毛滋养层细胞的分离纯化及马鞭草抗早孕机理的初步研究

目的 :探讨马鞭草抗早孕的细胞学作用机理。方法 :正常妊娠 6～ 8周早期胎盘 Percoll梯度离心分离出滋养层细胞进行体外培养 ,观察马鞭草对培养的滋养层细胞形态及绒毛膜促性腺激素分泌功能的影响。结果 :2 5、50、mg/ ml马鞭草乙醇提取液对滋养层细胞生长及绒毛膜促性腺激素分泌有明显的抑制作用。结论 :一定浓度的马鞭草可直接杀伤滋养层细胞 。