靶向HER2胞外结构域Ⅳ的单克隆抗体在乳腺癌中的应用进展

人表皮生长因子受体2(HER2)阳性乳腺癌侵袭性强且易转移,抗HER2靶向药物的应用能显著改善HER2阳性乳腺癌患者的预后。在已上市的HER2靶向药物中,靶向HER2胞外结构域Ⅳ的大分子单克隆抗体是治疗HER2阳性乳腺癌的基础靶向药物,主要包括曲妥珠单抗、伊尼妥单抗和马吉妥昔单抗。曲妥珠单抗用于乳腺癌全线治疗,循证医学证据充分,实践经验充足且安全性可控;伊尼妥单抗与曲妥珠单抗在HER2阳性转移性乳腺癌和新辅助/辅助治疗中疗效相似,且安全性可控;马吉妥昔单抗聚焦于携带CD16A-158F等位基因的患者,是晚期乳腺癌后线治疗的选择。临床上需根据患者具体病情选择最适合的药物。

Glycosylation-independent binding to extracellular domains 11-13 of mannose-6-phosphate/insulin-like growth factor-2 receptor mediates the effects of soluble CREG on the phenotypic proliferation of vascular smooth muscle cells

Background The present study aimed to investigate the detailed mode and specific sites for their binding as well as the functional relevance of this binding in the phenotypic proliferation of vascular smooth muscle cells(SMCs). Methods CREG knocked-down SMCs were employed to evaluate the biological activity of wtCREG and mCREG.Expressions of SMC differentiation markers SM myosin heavy chain(SM-MHC),SM-actin,heavy caldesmon and myocardin were determined by Western blotting using specific antibodies. Cellular growth of SMCs was assessed by bromide dewuridine (BrdU) incorporation and cell cycle analysis on fluorescence-activated cell sorting(FACS).A solid-phase binding assay was used to study the binding of CREG to extracellular domains of M6P/IGF2R.The cellular co-localization of the two recombinant CREGs with M6P/IGF2R was detected on SMC surface by immunoprecipitation and immunofluorescence analysis.Results The molecular weight of wtCREG was around 30 kD while that of the mCREG was～25 kD.Treatment of wtCREG with PNGase F reduced its molecular weight from～30 kD to～25 kD,whereas PNGase F treatment had no effect on the molecular weight of mCREG.Both wtCREG and mCREG proteins enhanced SMC differentiation,inhibited BrdU incorporation,and arrested cell cycle progression when added to the culture medium.In CREG knocked-down SMCs,the amount of CREG detected by immunoblotting in M6P/IGF2R immunoprecipitates was significantly reduced when compared to normal cells.Both recombinant CREGs co-immunoprecipitated with M6P/IGF2R, although slightly reduced amount of the mutant CREG was detected in M6P/IGF2R immunoprecipitates.Immunostaining revealed that His-tagged CREGs co-localized with IGF2R on the cell surface in a glycosylation-independent manner.In vitro binding assay showed that CREGs bound to M6P/ IGF2R extracellular domains 7-10 and 11-13 in a glycosylation -dependent and -independent manner,respectively.Further blocking experiments using soluble M6P/IGF2R fragments and M6P/IGF2R neutralizing antibody indicated that the biological activities of recombinant CREGs in SMC growth and the up-regulation of SMC differentiation markers were all abolished by treatment with the M6P/IGF2R neutralizing antibody. However,although the growth inhibitory effect of wtCREG was nearly abolished by D7-10 or D11-13,the effect of mCREG was only reversed by Dll-13,indicating that the binding to domains 11-13 is required for CREG to modulate the proliferation of SMCs.Conclusions These data suggest that solubleCREG proteins can exert their biological function via binding to the extracellular domains 7-10 and 11-13 of cell surface M6P/IGF2R in both a glycosylation-dependent and -independent manner.

Enhanced immuno-detection of shed extracellular domain of HER-2/neu

HER-2/neu oncogene is over-expressed and amplified in patients associated with metastatic breast cancer. An increased level (>15 ng/mL) in the shed extracellular domain (sECD-HER 2/neu) is indicative of the potential presence and as-sociated progression of this disease. A fluo-rescent ELISA incorporating the newly devel-oped ALYGNSA antibody-orientation system revealed a 10-fold increase in sensitivity (≤0.63 ng/mL) of sECD-HER 2/neu when compared to a control standard ELISA kit (≤7.5 ng/mL). This enhanced mode of detection has the potential to not only address breast and other cancers per se but also permit an in depth evaluation of “shed extracellular domains”, in general, and the role of these “proteolytic derived factors” in physiological signalling at normal levels.

Eukaryotic expression, purification and activity characterization of human soluble DSG2 extracellular domain protein

Objective:To construct a secretory eukaryotic expression vector of DSG2 fused with the Fc region of the human IgG,to validate its expression in 293T cells,and to purify the secretory protein with biological activity.Methods:The DSG2 extracellular domain fragment gene(DSG2ex),was amplified by PCR,and was inserted into the eukaryotic expression plasmid pCMV3-IgG1 to construct the recombinant eukaryotic expression plasmid-pCMV3-DSG2ex-IgG1.The successfully constructed eukaryotic expression plasmid was transfected into 293T cells to express and secrete DSG2 extracellular domain protein.The targeted protein was purified from the cell culture supernatant by Protein A affinity chromatography and confirmed by Western Blotting and ELISA.Results:The pCMV3-DSG2ex-IgG1 eukaryotic expression plasmid was successfully constructed.The highest protein expression level was obtained with 293T cells after 96 h of transfection.The relative molecular mass of the purified product was between 100 and 130 kDa was estimated by SDS-PAGE,which was consistent with the expectation.The yield of the purified protein reached 0.8 mg/ml with a purity over 90%.The purified DSG2 extracellular domain protein with IgG1 tag was recognized by IgG monoclonal antibodies by Western blotting.Moreover,the ELISA results showed that the prepared DSG2 extracellular domain protein had significant binding activity to human type 55 adenovirus Fiber Knob protein(HAdV-55).Conclusion:A simple and efficient method for eukaryotic expression and purification of human soluble DSG2 extracellular domain protein was successfully established,and biologically active DSG2 extracellular domain protein was purified,which laid the foundation for the later study of its protein function and anti-adenovirus drugs.

黄芪甲苷Ⅳ通过抑制TIM-1信号通路增加Th1/Th2细胞比率减轻IgA肾病小鼠肾损伤

目的探讨黄芪甲苷Ⅳ(AS-Ⅳ)对IgA肾病(IgAN)小鼠1型辅助T(Th1)细胞/Th2细胞平衡的影响及其可能作用机制。方法建立BALB/c小鼠IgAN模型,造模成功小鼠随机分为模型组、AS-Ⅳ低、中和高剂量组各10只,另设对照组10只。AS-Ⅳ低、中和高剂量组小鼠灌胃(12.5、25、50)mg/kg AS-Ⅳ混悬液(生理盐水配制),对照组及模型组给予等量生理盐水。测定各组小鼠24 h尿蛋白(24 hUPr)含量和尿红细胞计数;测定小鼠血尿素氮(BUN)、血清肌酐(Scr)和白蛋白(ALB)水平;ELISA检测各组小鼠血清γ干扰素(IFN-γ)、白细胞介素4(IL-4)和IL-10水平;流式细胞术检测小鼠外周血Th1/Th2细胞比率;HE染色观察小鼠肾组织病理学变化;反转录PCR和Western blot法分别检测小鼠肾组织中T细胞免疫球蛋白和黏蛋白结构域1(TIM-1)、Toll样受体4(TLR4)的mRNA和蛋白表达。结果与模型组比较,AS-Ⅳ低、中和高剂量组小鼠第12周和第15周尿红细胞计数、24 h UPr、BUN、Scr、IL-4、IL-10水平、Th2细胞比例、TIM-1与TLR4 mRNA和蛋白表达水平均明显降低,ALB、IFN-γ水平、Th1细胞比例和Th1/Th2细胞比率升高,且以AS-Ⅳ高剂量组效果最佳。结论AS-Ⅳ通过抑制TIM-1信号通路,增加Th1/Th2细胞比率,抑制炎症反应,减轻IgAN小鼠肾损伤。

慢性肾小球肾炎血、尿Ⅳ型胶原及尿黏蛋白的改变与肾脏病理关系初探

目的:观察肾功能正常的慢性肾炎患者的血、尿Ⅳ型胶原(Col-Ⅳ)及层黏蛋白(LN)含量的变化与肾脏病理改变的关系及临床应用价值。方法:(1)采用双抗体夹心酶联免疫吸附(ELISA)法测定67例肾功能正常的慢性肾炎患者和20例健康人的血、尿Col-Ⅳ与LN含量。(2)慢性肾炎患者均接受肾活检病理检查。观察以上指标与肾脏病理改变的关系。结果:(1)与健康人相比,慢性肾炎组患者血、尿Col-Ⅳ及LN水平均明显增高(P<0.05)。(2)系膜细胞增生Ⅲ级组、Ⅳ级组与健康人组比较,血、尿Col-Ⅳ及LN均明显增高(P<0.05)。系膜细胞增生程度与血Col-Ⅳ水平关系最密切(P<0.05)。(3)各系膜基质增生组与健康组比较,血、尿Col-Ⅳ及LN均显著增高(P<0.05)。系膜基质增生程度与尿Col-Ⅳ水平关系最为密切(P<0.05)。(4)肾小球球性硬化10%～25%组与健康人比较,血、尿Col-Ⅳ及LN均明显增高(P<0.05)。硬化率与血LN关系最密切(P<0.05)。(5)间质纤维化程度与尿Col-Ⅳ水平关系最密切(P<0.01)。(6)小管萎缩≤10%者较健康者,尿Col-Ⅳ、LN均显著增高(P<0.01)。小管萎缩>5%者较健康者,血Col-Ⅳ明显增高(P<0.01)。小管萎缩>10%者尿Col-Ⅳ则明显降低(P<0.05)。(7)血Col-Ⅳ水平与血LN水平正相关(P<0.01)。尿Col-Ⅳ水平与尿LN水平正相关(P<0.01)。但血、尿Col-Ⅳ水平之间及血、尿LN水平之间均无线性相关关系。结论:(1)肾功能正常的慢性肾炎患者血、尿Col-Ⅳ与LN水平显著高于健康人群。(2)血与尿Col-Ⅳ、LN水平的变化可在一定程度上反映肾脏病理的改变,与系膜细胞基质的增生程度、间质纤维化、肾小球球性硬化有一定的关系。但血Col-Ⅳ、LN水平主要反映了Col-Ⅳ、LN代谢的活跃,与系膜细胞增生关系更为密切;而尿Col-Ⅳ、LN水平则与基质增生、间质纤维化关系更为密切。它们之间均存在着相关关系。因此监测血与尿Col-Ⅳ、LN的动态变化,综合判断,对于监测肾脏纤维化倾向有一定价值。

血清Ⅳ型胶原测定在肝、肾疾病中的意义

用单克隆抗体酶免疫法分别检测５０例及９０例不同病期肝、肾疾病患者血清Ⅳ型胶原（ＣＬ－Ⅳ）水平。旨在探讨作为细胞外基质成分ＣＬ－Ⅳ在这两类疾病发展及硬化过程中变化的意义。发现血清ＣＬ－Ⅳ在肝、肾疾病中有不同程度改变，并与疾病严重程度密切相关。提示ＣＬ－Ⅳ代谢变化可能在肝、肾疾病进行性发展及组织硬化过程中起重要作用。血清ＣＬ－Ⅳ浓度可作为临床监测和判断患者肝、肾功能损害程度、活动状态及组织硬化的一项常规辅助指标。

Ⅳ型胶原在肾积水中的表达及意义

目的 :研究Ⅳ型胶原在肾积水中的表达及意义 ,并探讨其沉积与小管间质纤维化程度的相关性。方法 :采用免疫组织化学方法 (S P法 ) ,检测Ⅳ型胶原在 31例肾积水和 1 3例正常肾组织中的表达情况。结果 :Ⅳ型胶原在积水肾肾小管胞浆和肾间质表达明显增高 ,积水肾与正常肾组织中的光密度值分别为 0 .2 2 75± 0 .0 0 1 9和0 .1 6 4 0± 0 .0 0 1 3,差异有显著性 (P <0 .0 5 )。Ⅳ型胶原与间质纤维化病变程度呈正相关 (r=0 .6 31 4 ,P <0 .0 5 )。结论 :Ⅳ型胶原沉积可能造成小管功能改变 。

Ⅳ型胶原蛋白与肾脏疾病

Ⅳ型胶原蛋白作为肾脏基底膜中的支架结构,在维持肾脏滤过屏障中起着关键作用,其含量、分布和结构变化与肾脏疾病的发生发展密切相关。肾脏中IV型胶原蛋白的缺失和过度表达都将导致肾脏基底膜结构和功能异常,诱发或促进肾脏疾病的发生。因此,IV型胶原蛋白可能作为治疗靶点为临床肾脏疾病的控制提供新的策略。本文综述了IV型胶原蛋白在肾脏疾病中的作用。

Reg Ⅳ基因缺失CRD结构域片段获得及其表达载体的构建与转染

目的:探讨应用基因重叠延伸拼接PCR(SOE-PCR)技术构建Reg Ⅳ基因缺失CRD结构域表达载体,并转染Reg Ⅳ低表达结直肠癌细胞系。方法:应用SOE-PCR法获得Reg Ⅳ缺失CRD结构域片段,构建真核表达载体并转染Reg Ⅳ低表达结直肠癌LoVo细胞,G418筛选,RT-PCR检测鉴定。结果:经酶切鉴定筛选出的重组体测序结果与目的序列完全一致,重组载体构建成功,经pcDNA3.1-Reg Ⅳ-dom ain△转染的LoVo细胞Reg Ⅳ-dom ain△呈阳性表达。结论:利用SOE-PCR技术可成功构建Reg Ⅳ基因缺失CRD结构域的表达载体。

慢性肾炎血瘀证血尿Col-Ⅳ LN的改变及丹参注射液的作用初探

目的:观察肾功能正常的慢性肾炎血瘀证患者的血、尿Ⅳ型胶原(Col-Ⅳ)及层粘蛋白(LN)含量的变化与中医本虚证、血瘀证症状积分的关系及临床应用价值;观察复方丹参注射液治疗前后的血、尿Col-Ⅳ及LN含量的变化,探讨复方丹参注射液治疗肾脏纤维化的疗效及可能机制。方法:采用双抗体夹心酶联免疫吸附(ELISA)法测定67例肾功能正常的慢性肾炎血瘀症患者和20例健康人的血、尿Col-Ⅳ与LN含量,观察以上指标与中医本虚证及血瘀证症状积分的关系;67例慢性肾炎患者随机分为35例复方丹参治疗组和32例对照组,对照组给以潘生丁、雷公藤多苷等常规处理,伴肾病综合征者加用激素,血压高者加用降压药,治疗组给予以上对照组治疗+复方丹参注射液50mL静脉滴注。比较治疗前后两组的血、尿Col-Ⅳ及LN含量的变化。结果:与健康人相比,慢性肾炎组患者血、尿Col-Ⅳ及LN水平均明显增高(P<0.05);各本虚证型血、尿Col-Ⅳ及尿LN较健康者均明显增高(P<0.01),气阴两虚与健康者相比,血LN明显增高(P<0.01),气阴两虚与肺肾气虚比较,血Col-Ⅳ及血、尿LN均明显增高(P<0.05),脾肾阳虚与肝肾阴虚比较,尿Col-Ⅳ明显下降(P<0.01);各血瘀证组与健康人组比较,血、尿Col-Ⅳ及LN均明显增高(P<0.05,P<0.01),而各血瘀证组间两两比较,各指标均无显著差异,Spearm an相关分析结果显示,血、尿Col-Ⅳ与LN水平与血瘀证积分均无线性相关关系;治疗组治疗前后血Col-Ⅳ、LN及尿Col-Ⅳ、LN均明显下降(P<0.05)。治疗组与对照组治疗前后血Col-Ⅳ、LN及尿Col-Ⅳ、LN差值比较有显著差异(P<0.05)。Spearm an相关分析:治疗前后血Col-Ⅳ与血LN二者水平的改变呈显著正相关(P<0.01)。结论:肾脏纤维化可能是慢性肾炎血瘀证的内在物质基础,肾脏纤维化是肾脏局部的血瘀状态,即所谓的微型癥积。外在的血瘀证症状积分难于体现肾脏局部的瘀血严重程度。复方丹参注射液对于减轻慢性肾炎的纤维化程度,延缓纤维化进展可能有一定的益处,其抗肾脏纤维化作用可能是通过多个途径而实现的。对延缓肾脏纤维化的治疗提供了又一药物选择。

肾小球疾病患者血清Ⅳ型胶原测定的临床意义

本文应用单克隆抗体免疫法检测了53例健康人及50例不同病期的肾小球疾病患者血清Ⅳ型胶原水平,并与肾活检组织病理所见进行了比较。结果显示,肾功能受损害者血清Ⅳ型胶原水平明显高于正常人,且与肾单位损害的严重程度密切相关.提示Ⅳ型胶原的代谢变化在肾小球疾病进行性发展过程中起着重要作用.血清Ⅳ型胶原水平的测定,可以作为临床监测肾小球疾病活动及病程进展的有用指标。

Ⅲ型、Ⅳ型胶原在慢性胰腺炎组织中的表达

目的检测Ⅲ、Ⅳ型胶原在CP及正常胰腺组织中的表达水平,研究其在胰腺间质纤维化形成中的作用。方法免疫组织化学方法检测16例CP标本及6例正常胰腺组织中Ⅲ、Ⅳ型胶原的表达。结果16例CP中,Ⅲ型、Ⅳ型胶原表达均为轻度以上深染,其中重度深染50%（8/16）,中度深染31.25%（5/16）;而正常胰腺组织Ⅲ、Ⅳ型胶原表达均为浅染。正常胰腺组织中Ⅲ、Ⅳ型胶原表达于基底膜、间质纤维、导管壁、血管壁,Ⅲ型胶原以间质纤维表达最明显,Ⅳ型胶原以基底膜表达最明显。CP组织中Ⅲ型胶原表达于基底膜、间质纤维、导管壁、血管壁,以间质纤维最明显;Ⅳ型胶原表达于基底膜、间质纤维、导管壁、血管壁,以基底膜最明显。结论Ⅲ、Ⅳ型胶原的表达增强在胰腺纤维化的形成中可能有重要作用。

AMPK在高糖诱导大鼠肾小球系膜细胞Ⅳ型胶原过度表达中的作用

目的观察高糖环境下大鼠肾小球系膜细胞Ⅳ型胶原蛋白表达水平的变化,以及这种变化与AMP活化蛋白激酶(AMPK)的关系。方法实验分4组:对照组(糖浓度5.6 mmol/L)、高糖组(22.0 mmol/L)、低浓度5-氨基-4-甲酰胺咪唑核糖核苷酸(AICAR)组(0.5 mmol/L AICAR+高糖)和高浓度AICAR组(1.0 mmol/L AICAR+高糖)。孵育24 h后,用RT-PCR法测定AMPKα1mRNA水平,用Western blot法分别测定总AMPKα蛋白(AMPK)、磷酸化AMPKα蛋白(p-AMPK)和Ⅳ型胶原蛋白α5(COL4α5)亚单位的表达水平。结果高糖组AMPKα1mRNA水平低于对照组(P<0.01);高糖组总AMPKα蛋白和磷酸化AMPKα蛋白表达水平均低于对照组(P<0.01),高糖组COL4α5亚单位表达水平高于对照组(P<0.01);AMPK激活剂AICAR可在不同程度上纠正上述变化。结论高糖环境下大鼠肾小球系膜细胞Ⅳ型胶原蛋白表达水平上调,这可能与AMPK表达下调及其活性降低有关。

Extracellular and cytoplasmic regions of LRIG1 play a negative role in EGFR activity: Findings of a radioligand-binding assay

Objective Leucine-rich repeats and immunoglobulin-like domains 1(LRIG1) is a newly identified human gene that inhibits the epidermal growth factor receptor(EGFR), which on combining with a ligand, can drive tumor growth. This study investigated the interaction between human LRIG1 and EGFR and attempted to delineate the functions of as well as the mechanisms used by the extracellular(ECD) and cytoplasmic(CPD) domains of the human LRIG1 protein to downregulate human EGFR signaling activity.Methods Two constructed chimeric eukaryotic expression vectors, pIRES2-EGFP-3XFLAG-LRIG1-ET and p3FLAG-LRIG1-TC, encoding the extracellular and transmembrane regions(LRIG1-ET) and the transmembrane and cytoplasmic regions(LRIG1-TC), respectively, and the plasmid p3XFLAG-CMV-9-LRIG1 encoding full-length LRIG1(LRIG1-FL) were transfected into the human glioma cell line U251 or primary astrocytoma cells by using liposomes. The number and affinity of cell surface EGFR on transfected cells was determined by ^(125)I-EGF binding assay. Results The dissociation constant(KD) values for EGFR were higher, and the maximum increase was observed in the cells transfected into LRIG1-ET(1.36 folds). The number of maximal binding sites(Bmax) of the receptors was decreased in all transfected cells; the maximum decrease was noted in the cells transfected into LRIG1-FL(40.05%).Conclusion Both the ECD and CPD of LRIG1 are important to negate EGFR signaling. The ECD may interfere with the binding between EGFR and its ligand and facilitate the functions of CPD. The CPD may, when brought in proximity to EGFR, enhance receptor degradation. These two mechanisms can contribute to the downregulation of EGFR-mediated signaling by LRIG1.

海南捕鸟蛛毒素-Ⅳ在大肠杆菌中的分泌表达及纯化

海南捕鸟蛛毒素-Ⅳ(hainantoxin-Ⅳ,HNTX-Ⅳ)是从海南捕鸟蛛(Selenocosmia hainana)的毒液中分离得到的一种可以特异性抑制河豚毒素敏感型(TTX-S)钠通道的多肽毒素,并且能够选择性抑制Nav1.7亚型电压门控钠离子通道。HNTX-Ⅳ的成熟肽含有35个氨基酸残基,其结构通过3对二硫键稳定。HNTX-Ⅳ是研究钠通道结构和功能以及镇痛药物开发过程中非常有用的一种分子探针,但是其在天然毒素中的含量较少,很难分离足够量的组分进行后续研究。在本研究中,我们通过OEPR克隆构建了HNTX-Ⅳ的大肠杆菌分泌表达质粒pSE-G1M5-SUMO-HNTX-Ⅳ。将质粒pSE-G1M5-SUMO-HNTX-Ⅳ转化到大肠杆菌BL21(DE3)中进行自动诱导分泌表达,含有6×His标签和SUMO标签的融合蛋白质6×His-SUMO-HNTX-Ⅳ成功分泌到大肠杆菌的细胞外培养基中。通过弱阳离子交换柱富集和Ni-NTA柱纯化之后,成功获得了纯度较高的融合蛋白质6×His-SUMO-HNTX-Ⅳ。通过Ulp1激酶切割,重组HNTX-Ⅳ(rHNTX-Ⅳ)被释放出来,并通过RP-HPLC分离获得。通过MALDI-TOF质谱鉴定rHNTX-Ⅳ分子量为3.9876kD。通过膜片钳技术,10μmol/L的rHNTX-Ⅳ能够抑制90%以上的hNav1.7的电流,其IC_(50)值为126 nmol/L。本研究成功将HNTX-Ⅳ分泌到了大肠杆菌的细胞外培养液中,并最终获得了纯度较高且具有生理活性的rHNTX-Ⅳ分子,丰富了HNTX-Ⅳ的制备方法,为其后续研究奠定了基础。

非洲猪瘟病毒CD2v蛋白胞内域与胞外域的原核表达及其抗原性分析

【目的】应用大肠杆菌表达系统表达非洲猪瘟病毒(African swine fever virus,ASFV)CD2v蛋白胞外域(N-端,CD2v-N)与胞内域(C-端,CD2v-C)并分析两者的抗原性,为ASFV检测方法的研发提供试验依据和指导。【方法】构建CD2v-N和CD2v-C的重组原核表达质粒,在体外表达并纯化CD2v-N和CD2v-C蛋白,通过Western blotting对表达蛋白进行鉴定;用表达的CD2v-N和CD2v-C蛋白分别肌内接种免疫新西兰大白兔,共免疫3次,每次间隔2周;每次免疫后14 d,应用ELISA方法测定CD2v-N或CD2v-C的特异性抗体水平;用纯化后的CD2V-N和CD2v-C蛋白作为包被抗原,通过ELISA方法检测95份ASFV感染猪的血清CD2v-N或CD2v-C特异性抗体,比较CD2v-N和CD2v-C在猪体内诱导的免疫反应水平。【结果】重组蛋白CD2v-N和CD2v-C分别以包涵体和可溶性形式表达,分子质量分别为22.9和34.0 ku,均能与猪抗ASFV血清特异性结合;用CD2v-N蛋白首免家兔后14 d,血清中未检测到特异性抗体,而在CD2v-C首免的家兔血清中检测到了高滴度的特异性抗体;三免后14 d,CD2v-N和CD2v-C蛋白免疫家兔的血清特异性抗体效价分别为1∶125000和1∶107;ELISA检测结果显示,ASFV感染猪的血清中CD2v-C特异性抗体水平显著高于CD2v-N(P<0.05)。【结论】本研究表达了ASFV CD2v蛋白胞内域和胞外域,前者的抗原性比后者高,CD2v胞内域作为ASFV免疫学检测技术研究与开发的靶标更具优势。该研究结果对ASFV检测方法的研究与开发具有重要指导意义。

中性粒细胞胞外诱捕网通过CCDC25促进骨肉瘤细胞增殖、迁移和侵袭的作用研究

目的探究中性粒细胞胞外捕获网(neutrophil extracellular traps,NETs)在骨肉瘤细胞增殖、迁移和侵袭中的作用及其相关机制。方法纳入骨肉瘤患者和健康受试者各20例,通过ELISA检测血清中PAD4和H3cit水平。提取两组人群外周血中性粒细胞,比较NETs形成差异。将NETs与骨肉瘤细胞MG63共孵育,期间加入DNA降解酶DNaseⅠ,分为对照组、NETs组和NETs+DNaseⅠ组。通过蛋白质印迹检测CCDC25蛋白表达水平,CCK8检测细胞增殖水平,Transwell检测细胞迁移和侵袭水平。将si-NC和si-CCDC25转染至MG63,加入NETs共孵育,分为si-NC组和si-CCDC25组,通过蛋白质印迹检测CCDC25蛋白表达水平,CCK8检测细胞增殖水平,Transwell检测细胞迁移和侵袭水平。结果与健康受试者比较,骨肉瘤患者血清中PAD4和H3cit水平升高(P<0.05),NETs形成能力增强。与对照组比较,NETs组CCDC25蛋白表达升高,细胞增殖、迁移和侵袭水平升高(P<0.05)。与NETs组比较,NETs+DNaseⅠ组CCDC25蛋白表达降低,细胞增殖、迁移和侵袭水平降低(P<0.05)。与si-NC组比较,si-CCDC25组CCDC25蛋白表达降低,细胞增殖、迁移和侵袭水平降低(P<0.05)。结论NETs通过释放的DNA激活骨肉瘤细胞CCDC25表达,从而促进肿瘤细胞增殖、迁移和侵袭。

异钩藤碱对大鼠急性胰腺炎细胞的炎症和凋亡改善及ERK信号通路调控作用

目的观察异钩藤碱(LSO)对大鼠急性胰腺炎(AP)细胞炎症和凋亡改善及ERK信号通路调控作用。方法将AR42J细胞分为6组,对照组正常培养,模型组、LSO组、抑制剂组、LSO+抑制剂组、LSO+激活剂组加入100 nmol/L雨蛙素制备AP细胞模型,LSO组制模后加入40μmol/L LSO,抑制剂组制模后加入10μmol/L U0126,LSO+抑制剂组制模后加入40μmol/L LSO和10μmol/L U0126,LSO+激活剂组制模后加入40μmol/L LSO和0.1μmol/L C16-PAF。采用ELISA法、EdU法及Hoechst 33258染色法分别测定细胞培养液中的炎症因子(TNF-α、IL-6、IL-8、IL-1β)、细胞增殖率和凋亡率,qPCR法测定细胞中NLRP3、斑点样蛋白(ASC)、半胱氨酸蛋白酶-1(Caspase-1)mRNA,WB法测定细胞中ERK 1/2、p-ERK 1/2、NLRP3、ASC、Caspase-1蛋白。结果与对照组比较,模型组细胞TNF-α、IL-6、IL-8、IL-1β、凋亡率、p-ERK 1/2蛋白及NLRP3、ASC、Caspase-1 mRNA和蛋白升高,增殖率降低(P均<0.05);与模型组比较,LSO组、抑制剂组细胞炎症因子(TNF-α、IL-6、IL-8、IL-1β)、凋亡率、p-ERK 1/2蛋白及NLRP3、ASC、Caspase-1 mRNA和蛋白降低,增殖率升高(P均<0.05);与LSO组比较,LSO+抑制剂组中U0126增强了LSO对细胞上述指标趋势的作用,而LSO+激活剂组中C16-PAF则逆转了LSO对细胞上述指标趋势的作用(P均<0.05)。结论LSO对大鼠急性胰腺炎细胞的炎症和凋亡有改善作用,可能通过调控ERK信号通路来实现。

小鼠抗寨卡病毒包膜蛋白胞外区(Eecto)单克隆抗体的制备

目的制备小鼠抗寨卡病毒(ZIKV)包膜蛋白胞外区(Eecto)单克隆抗体。方法首先构建ZIKV Eecto的原核表达质粒pET28a-ZIKV-Eecto,将其转化至大肠杆菌感受态BL21后,利用异丙基β-D-硫代半乳糖苷(IPTG)诱导表达。重组Eecto蛋白以包涵体形式表达,经过变性、复性和超滤获得纯化的蛋白。将Eecto蛋白3次免疫后,获得多克隆抗体血清,进行效价测定,并利用ZIKV prME真核表达质粒转染的HEK293T细胞进行Western blot法和免疫荧光法分析。取效价较高的小鼠脾脏制备脾细胞,与SP2/0骨髓瘤细胞融合,通过有限稀释法获取分泌抗体的杂交瘤细胞,并进一步制备腹水。对腹水进行抗体效价测定、亚类分析。以ZIKV同属病毒日本脑炎病毒(JEV)、黄热病病毒(YFV)、登革病毒1-4(DENV1-4)、蜱传脑炎病毒(TBEV)的Eecto为包被抗原,利用ELISA分析ZIKV单克隆抗体的交叉反应性,进一步对效价高、特异性强的抗体进行特异性分析。结果成功构建了原核表达质粒pET28a-ZIKV-Eecto,并获得纯化的Eecto蛋白,该蛋白具有良好的免疫原性;制备筛选得到1D6、4F11、4H7、4F8四株单克隆抗体,其中三株(1D6、4H7、4F8)为IgGκ型抗体,一株(4F11)为IgMκ,1D6腹水效价大于1∶108;其中1D6和4H7为ZIKV特异性抗体,与其他黄病毒无交叉反应。结论成功制备了小鼠抗ZIKV Eecto单克隆抗体,为后续建立ZIKV检测方法及致病机制研究提供了实验材料。