Forkhead Box q1 promotes invasion and metastasis in colorectal cancer by activating the epidermal growth factor receptor pathway

BACKGROUND Colorectal cancer(CRC)is an extremely malignant tumor with a high mortality rate.Little is known about the mechanism by which forkhead Box q1(FOXQ1)causes CRC invasion and metastasis through the epidermal growth factor receptor(EGFR)pathway.AIM To illuminate the mechanism by which FOXQ1 promotes the invasion and metastasis of CRC by activating the heparin binding epidermal growth factor(HB-EGF)/EGFR pathway.METHODS We investigated the differential expression and prognosis of FOXQ1 and HB-EGF in CRC using the Gene Expression Profiling Interactive Analysis(GEPIA)website(http://gepia.cancer-pku.cn/index.html).Quantitative real-time polymerase chain reaction(qRT-PCR)and Western blotting were used to detect the expression of FOXQ1 and HB-EGF in cell lines and tissues,and we constructed a stable lowexpressing FOXQ1 cell line and verified it with the above method.The expression changes of membrane-bound HB-EGF(proHB-EGF)and soluble HB-EGF(sHB-EGF)in the lowexpressing FOXQ1 cell line were detected by flow cytometry and ELISA.Western blotting was used to detect changes in the expression levels of HB-EGF and EGFR pathway-related downstream genes when exogenous recombinant human HB-EGF was added to FOXQ1 knockdown cells.Proliferation experiments,transwell migration experiments,and scratch experiments were carried out to determine the mechanism by which FOXQ1 activates the EGFR signaling pathway through HB-EGF,and then to evaluate the clinical relevance of FOXQ1 and HB-EGF.RESULTS GEPIA showed that the expression of FOXQ1 in CRC tissues was relatively high and was related to a lower overall survival rate.PCR array results showed that FOXQ1 is related to the HB-EGF and EGFR pathways.Knockdown of FOXQ1 suppressed the expression of HB-EGF,and led to a decrease in EGFR and its downstream genes AKT,RAF,KRAS expression levels.After knockdown of FOXQ1 in CRC cell lines,cell proliferation,migration and invasion were attenuated.Adding HB-EGF restored the migration and invasion ability of CRC,but not the cell proliferation ability.Kaplan–Meier survival analysis results showed that the combination of FOXQ1 and HB-EGF may serve to predict CRC survival.CONCLUSION Based on these collective data,we propose that FOXQ1 promotes the invasion and metastasis of CRC via the HB-EGF/EGFR pathway.

Epidermal growth factor receptor:a key manipulator in molecular pathways of malignant glioma

The epidermal growth factor receptor （EGFR） is a member of the ErbB/EGFR family, including EGFR/Herl, ErbB2/Her2, ErbB-3/Her3, and ErbB-4/Her4. EGFR exerts its effects through the receptor tyrosine kinase phosphorylation and activation of important downstream signaling pathways in normal and neoplastic cells, mainly the Ras GTPase/MAP kinase （MAPK）, STAT3, and phosphatidylinositide 3 kinase-AKT pathways. EGFR deregulation is common in malignant glioma, especially primary glioblastoma, and exists in three forms： gene overexpression （amplification）, autocrine effects of EGFR activation, and activating receptor mutation （EGFRvlII）. However, some EGFR abnormalities have also been found in low-grade gliomas, including the nuclear localization of EGFR, expression in the microfoci of anaplastic transformation, and association with neovascularization in the mesenchyma of the glioma, which suggests that some unknown EGFR-related mechanisms are possibly responsible for its central role in the initiation and progression of malignant glioma. Uncovering these mechanisms will have potential value in the development of radio- therapy, chemotherapy, and EGFR-targeted therapy for glioma.

Effects of (-)-Epigallocatechin gallate on some protein factors involved in the epidermal growth factor receptor signaling pathway

（-）-Epigallocatechin gallate （EGCG）, a major polyphenolic constituent of green tea, can inhibit activity of specific receptor tyrosine kinases （RTKs） and related downstream signal transduction pathways, resulting in the control of unwanted cell proliferation. The epidermal growth factor receptor （EGFR） signaling pathway is one of the most important pathways that regulates growth, survival,proliferation and differentiation in mammalian cells. This review addresses the effects of EGCG on some protein factors involved in the EGFR signaling pathway in a direct or indirect manner. Based on our understanding of the interaction between EGCG and these factors, and based on their structures, EGCG could be used as a lead compound for designing and synthesizing novel drugs with significant biological activity.

PD-L1和CD8在HER2阳性乳腺癌患者中的表达及其与病理参数相关性分析

目的通过评估程序性死亡受体配体1(programmed cell death-ligand 1,PD-L1)和分化群8(cluster of differentiation 8,CD8)在肿瘤微环境中的表达情况及其与患者临床病理特征的相关性,明确PD-L1和CD8在判断人表皮生长因子受体2(human epidermal growth factor receptor 2,HER2)阳性乳腺癌患者预后方面的作用。方法选取2016年10月至2018年10月山东省滕州市中心人民医院收治的HER2阳性乳腺癌患者65例,所有患者均为女性。癌组织切片经免疫组织化学方法标记PD-L1和CD8;收集患者的临床病理资料,包括年龄、组织学分级、P53、KI-67、雌激素受体、孕激索受体、肿瘤淋巴结转移分类(tumor node metastasis classification,TNM)分期在内的7项与预后相关的临床病理参数。分别分析PD-L1和CD8的表达是否和上述临床病理参数相关。结果PD-L1阳性表达率为21.5%,PD-L1阳性表达与组织学分级和TNM分期相关,差异有统计学意义(χ^(2)=6.250,P=0.044;χ^(2)=13.730,P=0.001);CD8阳性表达率为21.5%,CD8表达与组织学分级和TNM分期相关,差异有统计学意义(χ^(2)=8.023,P=0.018;χ^(2)=6.117,P=0.047)。结论PD-L1和CD8表达与乳腺癌组织学分级和TNM分期相关,可能是HER2阳性乳腺癌患者重要的预后标志物。

The potential mechanism of Isodon suzhouensis against COVID-19 via EGFR/TLR4 pathways

Corona Virus Disease 2019(COVID-19)has brought the new challenges to scientific research.Isodon suzhouensis has good anti-inflammatory and antioxidant stress effects,which is considered as a potential treatment for COVID-19.The possibility for the treatment of COVID-19 with I.suzhouensis and its potential mechanism of action were explored by employing molecular docking and network pharmacology.Network pharmacology and molecular docking were used to screen drug targets,and lipopolysaccharide(LPS)induced RAW264.7 and NR8383 cells inflammation model was used for experimental verification.Collectively a total of 209 possible linkages against 18 chemical components from I.suzhouensis and 1194 COVID-19 related targets were selected.Among these,164 common targets were obtained from the intersection of I.suzhouensis and COVID-19.Gene Ontology(GO)and Kyoto Encyclopedia of Genes and Genomes(KEGG)enriched 582 function targets and 87 target proteins pathways,respectively.The results from molecular docking studies revealed that rutin,vitexin,isoquercitrin and quercetin had significant binding ability with 3 chymotrypsin like protease(3CLpro)and angiotensin converting enzyme 2(ACE2).In vitro studies showed that I.suzhouensis extract(ISE)may inhibit the activation of PI3K/Akt pathway and the expression level of downstream proinflammatory factors by inhibiting the activation of epidermal growth factor receptor(EGFR)in RAW264.7 cells induced by LPS.In addition,ISE was able to inhibit the activation of TLR4/NF-κB signaling pathway in NR8383 cells exposed to LPS.Overall,the network pharmacology and in vitro studies conclude that active components from I.suzhouensis have strong therapeutic potential against COVID-19 through multi-target,multi-pathway dimensions and can be a promising candidate against COVID-19.

脓毒症合并急性肾损伤患者外周血TLR4、HMGB1、MFG-E8表达水平及临床意义

目的探讨脓毒症合并急性肾损伤患者外周血Toll受体4(TLR4)、高迁移率族蛋白box-1(HMGB1)、乳脂球表皮生长因子-8(MFG-E8)表达水平及临床意义。方法选取本院ICU收治的110例脓毒症患者,其中脓毒症合并急性肾损伤50例(SIAKI组),脓毒症不伴急性肾损伤60例(非AKI组),同时选取同期健康体检正常者50例(对照组),采用单因素方差分析3组患者TLR4、HMGB1、MFG-E8表达差异,采用Pearson分析三者表达相关性,进一步通过Logistic回归分析影响SIAKI严重程度的因素。结果 SIAKI组、非AKI组患者外周血TLR4、HMGB1表达水平明显高于对照组(P <0.05),且SIAKI组高于非AKI组(P <0.05),SIAKI组、非AKI组患者外周血MFG-E8表达水平低于对照组(P <0.05),SIAKI组低于非AKI组(P <0.05);SIAKI组患者C反应蛋白(CRP)、降钙素原(PCT)、血肌酐、尿素、尿酸及急性生理学与慢性健康情况评分系统Ⅱ(APACHEⅡ)评分显著高于非AKI组(P <0.05),肾小球滤过率(eGFR)明显低于非AKI组(P <0.05);SIAKI患者外周血TLR4、HMGB1水平与尿素、尿酸无相关性(P> 0.05),与CRP、PCT、血肌酐、eGFR、APACHEⅡ评分呈正相关(P <0.05);MFG-E8表达水平与CRP、尿素、尿酸无相关性(P>评分呈负相关(P <0.05);CRP、PCT、血肌酐、eGFR、TLR4、HMGB1是影响SIAKI严重程度的危险因素(P <0.05),MFG-E8是影响SIAKI严重程度的保护因素(P <0.05)。结论 SIAKI患者存在外周血TLR4、HMGB1水平升高,MFG-E8水平降低现象,TLR4、HMGB1、MFG-E8可作为SIAKI严重程度的检测指标。

血清TLR4、MFG-E8及HMGB1对脓毒症患者并发急性肾损伤的诊断价值

目的探讨外周血Toll样受体4(TLR4)、乳脂球表皮生长因子8(MFG-E8)及高迁移率族蛋白B1(HMGB1)水平对脓毒症患者并发急性肾损伤(AKI)的诊断价值。方法选择脓毒症患者130例,根据KGIDO标准将患者分为AKI组63例、非AKI组67例。采用ELISA法检测血清TLR4、MFG-E8、HMGB1,并收集相关指标。采用单因素和多因素Logistic回归分析脓毒症患者并发AKI的危险因素;采用受试者工作特征(ROC)曲线评价血清TLR4、MFG-E8、HMGB1水平对脓毒症患者并发AKI的诊断价值。结果AKI组血清TLR4、HMGB1水平高于非AKI组,血清MFG-E8水平低于非AKI组(P均<0.05)。AKI组序贯器官衰竭评分、基线血肌酐、基线eGFR、乳酸水平高于非AKI组,血清白蛋白水平低于非AKI组(P均<0.05);两组其他指标比较差异均无统计学意义(P均>0.05)。AKIⅢ期的脓毒症患者TLR4、HMGB1水平比较:AKIⅢ期>AKIⅡ期>AKIⅠ期;MFG-E8水平比较:AKIⅢ期<AKIⅡ期<AKIⅠ期。两两比较差异均有统计学意义(P均<0.05)。TLR4、HMGB1水平升高是脓毒症患者并发AKI的危险因素(OR均>1,P均<0.05),MFG-E8水平升高是脓毒症患者并发AKI的保护因素(OR>1,P<0.05)。TLR4、HMGB1及MFG-E8联合检测诊断脓毒血症患者并发AKI的曲线下面积大于三者单独检测(P均<0.05)。结论脓毒症并发AKI的患者血清TLR4、HMGB1水平升高,MFG-E8水平降低,三者水平变化可反映患者肾损伤程度,有助于脓毒症并发AKI的早期诊断。

表皮生长因子受体通路底物8疫苗对乳腺癌细胞的抑制效应及其可能机制

目的：探索表皮生长因子受体通路底物8（epidermal growth factor receptor substrate 8，EPS8）疫苗对乳腺癌细胞的抑制效应及其可能的机制。方法：Western blotting检测EPS8蛋白在小鼠乳腺癌4T1细胞株中的表达。通过基因重组、表达和纯化等技术制备特异性的小鼠源性EPS8，以EPS8蛋白为靶点制备抗肿瘤疫苗并免疫BALB/c小鼠，间接ELISA测定免疫前后不同时间小鼠血清内抗EPS8抗体效价；流式细胞术检测免疫前后的脾T淋巴细胞亚群比例。建立乳腺癌4T1细胞荷瘤小鼠模型并接种EPS8疫苗，接种佐剂作为对照，比较2组荷瘤小鼠的生存期、肿瘤体积、肿瘤重量，计算EPS8疫苗抑瘤率；流式细胞术检测荷瘤小鼠脾T淋巴细胞亚群比例，LDH法检测其细胞毒性T细胞（CTL）杀伤率。结果：EPS8蛋白在乳腺癌4T1细胞株中高表达。成功构建的EPS8蛋白疫苗免疫小鼠后产生抗EPS8抗体，且随着免疫次数的增加，小鼠体内抗EPS8抗体滴度呈上升趋势。乳腺癌4T1细胞接种于经EPS8疫苗或佐剂免疫后的小鼠后，与佐剂对照组相比，EPS8疫苗组小鼠生存期显著升高[中位生存时间：44（38~50） vs 37 （34~40） d; t=2.477, P=0.043]，肿瘤质量显著降低[（2.21±0.35）vs（3.31±0.88）g；t=3.574，P=0.009]，EPS8疫苗的抑瘤率为33.23%。EPS8疫苗组小鼠脾CD4＋T比例和CD4＋/CD8＋比值均显著高于佐剂对照组（P〈0.001），EPS8疫苗组CD4＋CD25＋Treg/CD4＋T细胞的比值显著低于佐剂对照组（P〈0.001）。效靶比为20〖DK〗∶1时，EPS8疫苗组CTL对靶细胞的杀伤活性即显著高于佐剂对照组[（19.05±4.41）% vs （13.36±3.10）%；t=2.263，P=0.040] 。结论：EPS8疫苗不仅具有诱导小鼠产生体液免疫应答的功能，还能够降低荷瘤小鼠体内Treg细胞比例，激活机体内T细胞免疫功能；EPS8疫苗可抑制肿瘤的生长、有效延长荷瘤小鼠的生存期。

ADAM8、EGFR在非小细胞肺癌中的表达及其相关性

背景与目的:去整合素-金属蛋白酶8(a disintegrin and metalloprotease 8,ADAM8)表达增高与肿瘤的发生、发展、侵袭、转移密切相关,但有关其在肺癌中的表达报道较少,尤其非小细胞肺癌(non-small cell lung cancer,NSCLC)中ADAM8与表皮生长因子受体(epidermal growth factor receptor,EGFR)相关性的研究目前尚未见报道。本研究旨在探讨ADAM8和EGFR在人NSCLC中的表达水平,并分析两者的相关性。方法:应用组织芯片(tissue microarray)结合免疫组化法(immunohistochemmistry)检测ADAM8与EGFR在49例肺癌组织、28例癌旁肺组织及13例肺良性病变组织中的表达情况,并分析两者的相关性及其与各病例的临床病理因素之间的关系。结果:ADAM8、EGFR蛋白的阳性表达主要定位在胞浆和胞膜。ADAM8、EGFR在NSCLC组织中的阳性率(73.5%、69.4%)显著高于癌旁组织(10.7%、14.2%)及肺良性病变组织(15.4%、23.1%)(P<0.01)。ADAM8、EGFR在鳞癌(73.1%、65.4%)与腺癌(80.0%、75.0%)的阳性率差异无统计学意义(P>0.05)。ADAM8、EGFR在N1-N3期NSCLC的阳性率(85.7%、82.8%)显著高于N0期NSCLC(42.8%、35.7%)(P<0.01)。ADAM8、EGFR在Ⅲ～Ⅳ期NSCLC(90.0%、90.0%)的阳性率显著高于Ⅰ～Ⅱ期(62.1%、65.5%)(P<0.05)。ADAM8和EGFR的表达具有一致性,Kappa值为0.522;两者表达呈正相关(r=0.589,P<0.01)。结论:ADAM8与EGFR在NSCLC组织中的表达均增高,两者具有较高的一致性。

表皮生长因子受体通路底物8、硫酸乙酰肝素酶以及基质金属蛋白酶在急性白血病的表达及其相关性研究

目的通过分析急性白血病(AL)患者骨髓液表皮生长因子受体通路底物8(EPS8)、硫酸乙酰肝素酶(HPSE)以及基质金属蛋白酶(MMP)表达水平,评估3种指标联合检测对患者病情及预后的预测价值。方法将2017年10月—2018年10月于内蒙古科技大学包头医学院第一附属医院血液科治疗的60例患者分为两组:急性白血病患者为实验组(AL组)和缺铁性贫血患者为对照组,每组30例。收集每组患者骨髓标本,应用RT-PCR法检测EPS8、HPSE以及MMP-2的mRNA表达水平,应用流式细胞检测技术检测骨髓细胞表面EPS8、HPSE以及MMP-2的表达水平。通过比较两组EPS8、HPSE以及MMP-2的表达水平,应用多因素Logistic回归分析进一步探讨急性白血病完全缓解与未缓解组的因子表达及其临床相关意义。结果急性白血病患者骨髓液中EPS8、HPSE以及MMP-2因子表达水平与对照组存在显著差异(均P<0.05);多因素Logistic回归分析显示,MMP-2、EPS8是随访1年患者是否完全缓解的影响因素(P<0.05)。结论急性白血病患者骨髓EPS8、HPSE以及MMP-2表达水平升高,且联合检测患者骨髓白血病细胞中EPS8、MMP水平能较好地评估AL患者的临床转归及预后。

血清TLR4及MFG-E8与子痫前期患者表达及发生早期肾损伤的关系

目的研究子痫前期患者外周血中TLR4和MFG-E8在子痫前期患者中的表达与诊断意义,并探讨其与子痫前期发生早期肾损伤的关系。方法用酶联免疫吸附法对妊娠期高血压患者30例,轻度子痫前期患者30例、重度子痫前期30例以及正常妊娠30例患者外周血中TLR4和MFG-E8表达水平。结果①外周血TLR4表达水平随病情加重呈逐渐升高趋势,sPE>mPE>GH>NP组;外周血MFG-E8表达水平随病情加重呈逐渐降低趋势,sPE<mPE<GH<NP组。TLR4和MFG-E8表达水平在多组间进行单因素方差分析及组间两两比较,均具有显著性差异(P<0.01)。②外周血TLR4与MFG-E8表达水平随着子痫前期病情进展呈负相关(r=-0.799,P=0.000);在子痫前期并发早期肾损伤的病例中,外周血TLR4与MFG-E8表达水平仍呈明显负相关(r=-0.875,P=0.000)。③外周血TLR4与MFG-E8表达水平诊断PE的敏感度分别为83.33%、78.33%,特异度分别为80.00%、86.67%;TLR4联合MFG-E8诊断PE的敏感度98.00%,特异度78.57%;TLR4、MFG-E8及TLR4联合MFG-E8诊断PE的ROC曲线下面积分别是0.850、0.889及0.928。结论TLR4与MFG-E8均密切参与子痫前期发病机制,且随病情进展,TLR4表达水平呈逐渐升高趋势,而MFG-E8则呈下降趋势,两者之间呈负相关。PE患者并发早期肾损伤时TLR4与MFG-E8负相关更明显。TLR4联合MFG-E8对诊断子痫前期的预测价值更高,为临床上子痫前期患者的早期诊断提高可靠依据。

Differential roles of EPS8 in carcinogenesis:Loss of protein expression in a subset of colorectal carcinoma and adenoma

AIM:To analyze the epidermal growth factor receptor pathway substrate 8(EPS8) expression status and role in colorectal carcinogenesis given that EPS8 has a conserved actin barbed-end capping function that is required for proper maturation in intestinal cells.METHODS:We studied 8 colon cancer cell lines and 58 colorectal tumors(19 adenomas and 39 carcinomas).We performed expression microarray analysis of colon cancer cell lines followed by loss of heterozygosity(LOH)analysis and immunohistochemistry for EPS8 expression in colon tumors.Subsequently,we performed mutation analysis by direct sequencing and methylation analysis by bisulfite sequencing and methylation-specific polymerase chain reaction assays.RESULTS:Expression microarray analysis of colon cancer cell lines showed overexpression of EPS8 transcript in all lines but RKO.Genome wide loss of heterozygosity(LOH) analysis of colon tumors,showed considerable LOH at the EPS8 gene locus.Immunohistochemically,EPS8 was constitutively expressed in normal colonic mucosa with a dot-like supranuclear localization with accentuation at the luminal surface supporting its proposed role in epithelial maturation.Nineteen colon tumors(4 adenoma,15 carcinoma) out of 51(37%) showed strikingly tumor specific EPS8 protein loss.Of the remaining tumors,5/51(2 adenoma,and 3 carcinoma,10%) showed marked overexpression,while 27/51 tumors(53%) showed retained expression.Mutation analysis revealed a missense mutation(c.794C>T,p.R265C) in exon 8 in RKO.The EPS8 promoter was also methylated in RKO,but there was no significant methylation in other cell lines or carcinoma specimens.CONCLUSION:The loss of EPS8 expression in colorectal adenomas and carcinomas suggests that down regulation of this gene contributes to the development of a subset of colorectal cancers,a finding which could have applications in diagnosis and treatment.

8-Br-cAMP联合顺铂作用于肺腺癌细胞A549的初步研究

目的:观察8-溴-环腺苷酸(8-Br-cAMP)联合顺铂(DDP)对人肺腺癌细胞A549生长及其表皮生长因子受体(EGFR)表达的影响。方法:MTT法测定不同浓度8-Br-cAMP、DDP以及两药联用处理人肺腺癌细胞A549后细胞增殖活性的差异;应用RT-PCR技术检测EGFR mRNA表达水平的变化;Western blot技术检测EGFR蛋白表达水平的变化;利用流式细胞术测定细胞周期的改变。结果:8-Br-cAMP及DDP均能抑制人肺腺癌细胞A549的增殖,并呈浓度及时间依赖性;DDP联合8-Br-cAMP细胞抑制率显著高于相应浓度单药组(P<0.05),两者呈现出相加的抗瘤效果。8-Br-cAMP可下调人肺腺癌A549细胞EGFR mRNA和蛋白的表达。8-Br-cAMP将细胞周期阻滞在G2/M期(P<0.05)。结论:8-Br-cAMP、DDP均可抑制A549细胞增殖。8-Br-cAMP可显著提高顺铂的细胞毒作用,增强化疗效果,并将细胞阻滞于G2/M期。8-Br-cAMP可以下调EGFR表达,可一定程度地逆转化癌细胞。

8-MOP、ATRA以及二者联合应用对Mc3细胞EGFR表达的影响

目的 :研究 8 -甲氧基补骨脂素 (8-Methoxypsoralen ,8-MOP)、全反式维甲酸 (AllTransRetinoicAcid ,ATRA)以及两者联合应用对粘液表皮样癌高转移克隆细胞株 (The 3rdCloneofMucoepidermoidCarcinomaCellLine - 1,Mc3)细胞表皮生长因子受体 (EpidermalGrowthFactorReceptor,EGFR)表达的影响。 方法 :免疫组织化学染色方法。结果 :EGFR表达分别为 :对照组 (+ + ) ;8-MOP组 (+ ) ;ATRA(+ ) ;8-MOP与ATRA联合用药组 (+ )。结论

顺铂作用下卵巢癌细胞株CP70中Eps8表达变化研究

目的:观察肿瘤相关抗原Eps8在卵巢癌细胞株A2780、CP70、SKOV3、SKOV3/DDP中的表达情况,筛查出Eps8高表达细胞株CP70。观察顺铂(DDP)作用下CP70细胞中Eps8在蛋白水平表达的变化,探讨Eps8在卵巢癌化疗耐药中的作用。方法:用实时荧光定量PCR法检测Eps8在卵巢癌细胞株中mRNA的表达水平,用Western blot法检测Eps8蛋白表达水平,筛选出高表达株CP70。用不同浓度DDP作用于CP70细胞24h、48h,用Western blot法检测Eps8在蛋白水平的变化。结果:随着药物浓度的增加及作用时间的延长,Eps8在蛋白水平的表达明显升高。结论:顺铂处理CP70细胞后,Eps8的蛋白表达量升高,且和DDP作用的时间及剂量有依赖性,即DDP可诱导CP70细胞中Eps8表达的上调。因此推测,Eps8在卵巢癌顺铂耐药形成机制中发挥重要作用。

柔红霉素对KG1a细胞增殖及肿瘤相关抗原Eps8表达的影响

本研究旨在观察柔红霉素(DNR)对KG1a细胞株的杀伤抑制作用及新型肿瘤相关抗原表皮生长因子受体通路底物8(Eps8)在KG1a细胞中的表达,在mRNA和蛋白水平探讨DNR作用于KG1a后对Eps8表达的影响。不同浓度DNR作用于KG1a细胞24、48和72 h,用台盼蓝拒染色法检测药物对KG1a细胞的杀伤抑制率,用实时荧光定量PCR法检测Eps8 mRNA转录水平的变化和Western blot法观察Eps8蛋白表达变化。结果表明:随着药物浓度(0.1,0.4μg/ml)的增加及作用时间(24,46,72 h)的延长,DNR对KG1a细胞的杀伤抑制率显著提高(r=0.983,P<0.01);不同DNR药物浓度作用于KG1a 24、48和72 h后,Eps8表达水平以DNR作用浓度和时间依赖方式明显下降(r=0.979,P<0.05)。结论:随药物浓度的增加和作用时间的延长,DNR对KG1a细胞的杀伤抑制率提高,使Eps8表达下降,推测降低Eps8的表达可能是DNR抑制KG1a细胞增殖的机制之一。

Eps8抗原改造表位HLA-A*0201限制性抗肿瘤能力观察

目的观察人表皮生长因子受体通路底物8(Eps8)抗原改造表位是否有人白细胞抗原A(HLA-A)*0201限制性抗肿瘤能力。方法替换Eps8抗原锚定位点氨基酸获得改造肽,用BIMAS、SYFPEITHI在线数据库及Aotodock 4.2软件预测改造表位与HLA-A*0201分子的结合力,筛选出稳定结合的改造表位E1-9V(ILDDIEFFV)、E1-1Y9V(YLDDIEFFV)。用经典肽结合力实验检测各改造表位与HLA-A*0201分子的亲和力。制备天然表位(E1)、E1-9V、E1-1Y9V特异性杀伤性T淋巴细胞(CTLs)。用乳酸脱氢酶(LDH)释放试验检测并比较E1-9V、E1-1Y9V特异性CTLs对MCF-7细胞、沉默Eps8的MCF-7细胞(MCF-7/shRNA)和抗HLA-A2抗体预孵育的MCF-7细胞(MCF-7/A2Ab)的杀伤率,E1-9V、E1-1Y9V特异性CTLs对SW480、U251、K562、IM-9细胞的杀伤率,E1、E1-9V、E1-1Y9V特异性CTLs对T2细胞的杀伤率。结果 E1-9V、E1-1Y9V均可与HLA-A*0201分子B、F对接口袋的氨基酸形成稳定氢键。肽结合力实验结果显示E1-9V、E1-1Y9V与HLA-A*0201均具有高亲和力,且高于天然表位E1,P均<0.05。E1-9V、E1-1Y9V特异性CTLs对MCF-7/shRNA、MCF-7/A2Ab细胞杀伤率明显低于MCF-7细胞,P均<0.05。E1-9V、E1-1Y9V特异性CTLs对SW480、U251细胞杀伤率明显高于K562、IM-9细胞(P均<0.05)。E1-1Y9V特异性CTLs对T2细胞的杀伤率显著高于E1、E1-9V特异性CTLs,P均<0.05。结论 Eps8抗原改造表位E1-9V、E1-1Y9V与天然表位E1相比具有更高的HLA-A*0201分子亲和力,保留了原有的免疫原性,并且E1-1Y9V抗肿瘤免疫效应强于天然表位E1。

8-氯腺苷抑制人胃癌细胞增殖相关信号蛋白的作用

目的探讨8-氯腺苷是否会影响肿瘤细胞的表皮生长因子受体(EGFR)及其相关信号蛋白的表达.方法人胃癌BGC-823细胞与不同浓度8-氯腺苷共孵育.SRB染色法观察细胞增殖;Western蛋白印迹法观察细胞增殖相关信号蛋白的表达.结果8-氯腺苷1.0, 2.5,5.0,7.5和10 μmol*L-1作用24 h,浓度依赖性抑制BGC-823细胞增殖,抑制率分别为19.7%,31.8%, 40.1%, 49.8%和56.7%.7.5 μmol*L-18-氯腺苷作用BGC-823细胞24, 48和72 h,抑制率分别为49.8%, 49.1%和45.6%.Western蛋白印迹结果表明,8-氯腺苷2.5～7.5 μmol*L-1作用24 h,BGC-823细胞EGFR蛋白表达减少;Raf-1蛋白表达变化不显著;p-MEK和p-ERK磷酸化蛋白表达增加.结论8-氯腺苷可抑制BGC-823细胞增殖;改变EGFR-Raf/MEK/ERK等一系列信号蛋白的表达可能是其抑制细胞增殖的重要途径之一.

miR-3074通过靶向EPS8基因对宫颈癌细胞增殖和侵袭的影响

目的探讨miR-3074通过靶向调节表皮生长因子受体通路底物8(epidermal growth factor receptor substrate 8,EPS8)基因表达对宫颈癌细胞增殖和侵袭的影响。方法应用OncoLnc在线数据库分析miR-3074表达水平与宫颈癌患者总生存期的关系。实时荧光定量聚合酶链反应(real-time fluorescence quantitative polymerase chain reaction,RT-qPCR)检测miR-3074在宫颈癌细胞系(SiHa、HCC94、C33A、HeLa)和正常宫颈上皮细胞H8中的表达。选取miR-3074表达最低的细胞系,分别转染对照模拟物(对照组)和miR-3074模拟物(miR-3074组)。CCK-8法和Transwell实验分别检测细胞增殖活力和侵袭能力。生物信息学软件RNAhybrid预测miR-3074的靶基因,双荧光素酶报告基因实验验证miR-3074与靶基因的靶向关系。qRT-PCR和Western blot法检测miR-3074对靶基因表达的影响。结果miR-3074表达水平较高的宫颈癌患者总生存期长于miR-3074表达水平较低的患者,差异有统计学意义(P<0.01)。与H8细胞比较,宫颈癌细胞系中miR-3074表达降低(P<0.05),miR-3074表达最低的细胞系是HCC94(P<0.01)。对照组和miR-3074组miR-3074表达分别为1.03±0.17和13.49±2.66,差异有统计学意义(P<0.01)。与对照组比较,miR-3074组HCC94细胞增殖活力降低(P<0.05),细胞侵袭能力降低(P<0.01)。miR-3074能作用于EPS8mRNA的3′非翻译区(P<0.01)。与对照组比较,miR-3074组EPS8基因表达显著降低(P<0.01)。结论miR-3074在宫颈癌细胞系中表达下调,miR-3074能够抑制宫颈癌HCC94细胞的增殖和侵袭,其机制可能与靶向抑制EPS8表达有关。

血清TLR4、TLR9、MFG-E8、UMOD判断急性胆囊炎不同严重程度的研究

目的研究血清Toll样受体(TLR)4、TLR9、乳脂球表皮生长因子8(MFG-E8)、尿调节素(UMOD)判断急性胆囊炎不同严重程度的价值。方法回顾性纳入2018年6月至2021年6月北京市应急总医院收治的98例急性胆囊炎患者作为研究对象,依据急性胆囊炎严重程度分为轻度组(n=35)、中度组(n=44)、重度组(n=19)。患者于入院24 h内检测血清TLR4、TLR9、MFG-E8、UMOD水平,以受试者工作特征(ROC)曲线分析血清TLR4、TLR9、MFG-E8、UMOD水平诊断重度急性胆囊炎的价值,以Pearson相关系数分析血清TLR4、TLR9、MFG-E8、UMOD水平与急性胆囊炎的相关性。结果3组血清TLR4、TLR9水平比较,重度组高于中度组,中度组高于轻度组;MFG-E8、UMOD水平比较,重度组低于中度组,中度组低于轻度组,差异均有统计学意义(P<0.05)。经ROC曲线分析,TLR4≥33.747 ng/mL、TLR9≥16.815 ng/mL、MFG-E8≤96.522 pg/mL、UMOD≤63.972 mg/mL是诊断重度急性胆囊炎的最佳截断值,曲线下面积分别为0.881、0.805、0.820、0.795,预测价值好(P<0.05)。经Pearson相关性分析,血清TLR4、TLR9与急性胆囊炎严重程度呈正相关(r=0.572、0.496,P<0.05),血清MFG-E8、UMOD水平与急性胆囊炎严重程度呈负相关(r=-0.591、-0.512,P<0.05)。结论随急性胆囊炎的加重,血清TLR4、TLR9水平逐渐升高,血清MFG-E8、UMOD水平逐渐降低,对于诊断重度急性胆囊炎具有较好的价值,可将TLR4≥33.747 ng/mL、TLR9≥16.815 ng/mL、MFG-E8≤96.522 pg/mL、UMOD≤63.972 mg/mL作为诊断重度急性胆囊炎的参考指标。