重组人睫状神经营养因子的聚乙二醇化修饰简

目的：研究重组人睫状神经营养因子（rhCNTF）突变体的聚乙二醇（PEG）化修饰,对rhCNTF的PEG化产物进行初步分离纯化及相关生物活性检测。方法：采用分子生物学技术经点突变得到rhCNTF的突变体cNm通过实验设计研究CN10的最佳PEG化条件;采用分子筛层析方式对偶联产物进行初步纯化,最后用ELISA和小鼠体重增长抑制法检测PEG化后的CN。。蛋白的生物活性。结果：能运用mPEG—MAL对CN,。进行定点修饰,PEG化后用Superdex200能够分离CN10;PEG化后的CN10每2d腹腔注射1次,对小鼠体重的增长抑制率可达50％,与rhCNTF每天注射2次的体重增长抑制作用相当。结论：CN10蛋白在PEG化修饰后,其减重效应持续时间明显延长。     

人白细胞介素11的定点聚乙二醇修饰

利用人白细胞介素11（hIL-11）无半胱氨酸（Cys）残基这一特点,通过定点突变将一个Cys残基引入hIL-11的N末端。然后,利用与Cys 巯基特异性反应的mPEG-马来酰亚胺将mPEG偶联到预先选定的位点,经层析纯化得到hIL-11的定点PEG修饰物。利用依赖型细胞株7TD1测定其生物学活性,结果表明,其体外生物学活性保持原有hIL-11活性的30%左右。定点聚乙二醇修饰方法为定向改造hIL-11,提高其药效的应用研究打下基础。     

重组人白细胞介素－6与肿瘤坏死因子突变体融合蛋白的构建及表达

针对肿瘤坏死因子（ＴＮＦ）在肿瘤治疗剂量下产生的严重毒副作用及一些肿瘤细胞上白细胞介素－６（ＩＬ－６）受体明显增高的事实,根据ＴＮＦ结构与功能研究的最新信息,利用ＰＣＲ技术,对人ＴＮＦα基因进行了改造,并将其与人ＩＬ－６成熟肽编码区ｃＤＮＡ通过人工接头进行融合。融合蛋白在大肠杆菌中表达后,Ｗｅｓｔｅｒｎｂｌｏｔ分析表明,分子量约为３７ｋＤ;活性检测结果证实,该融合蛋白兼具有ＴＮＦ抗肿瘤活性和结合ＩＬ－６受体的能力,在高表达ＩＬ－６受体的人骨髓瘤细胞上测得的细胞毒活性较同样位点突变的ＴＮＦ高约３倍。     

中国白兔白介素-10基因的克隆、表达及其抗体的制备

目的克隆并表达中国白兔IL-10基因,制备抗IL-10多克隆抗体。方法运用RT-PCR对从ConA诱导后的中国白兔外周血单核细胞(PMBCr)总RNA中扩增IL-10基因,克隆后进行测序和遗传进化分析,同时将其亚克隆pET28a中,在大肠杆菌中诱导表达,并用纯化的表达产物制备多克隆抗体。结果该基因全长537 bp,编码178个氨基酸。与欧洲兔IL-10基因同源性很高,但与鼠、鸡、河豚和斑马鱼等不同物种IL-10基因差异较大。经IPTG诱导后,重组菌体裂解物经SDS-PAGE电泳可检测到相对分子质量为23.4×103的重组蛋白。Western blot分析表明,中国白兔IL-10基因已经表达。重组表达的蛋白量可占菌体蛋白的15.2%。结论成功实现了中国白兔IL-10的原核表达,制备了小鼠抗兔IL-10的多克隆抗体。     

粒细胞—巨噬细胞集落刺激因子／白细胞介素—3融合蛋白的表达研究

利用ＰＣＲ扩增得到粒细胞－巨噬细胞集落刺激因子（ＧＭ－ＣＳＦ）、白细胞介素－３（ＩＬ－３）完整基因片段,将其分别克隆ｐＧＥＭ－Ｔ构建成ＧＭ－ＣＳＦ／ＩＬ－３融合蛋白基因,ＤＮＡ序列与设计预期一致。将得到的融合蛋白基因克隆对７２ＲＮＡ聚合酶表达载体ｐＴ７ｚｚ,得到表达质粒ｐＦｕ,经转化至表达宿主Ｅ．ｃｏｌｉ ＢＬ２１（ＤＥ３）,在ＩＰＴＧ诱导下获得融合蛋白目的产物的直接表达。经ＳＤＳ－ＰＡＧＥ电泳鉴     

粒细胞-巨噬细胞集落刺激因子/白细胞介素-3融合蛋白的表达研究

利用PCR扩增得到粒细胞巨噬细胞集落刺激因子(GM-CSF)、白细胞介素-3(IL-3)完整基因片段,将其分别克隆至pGEM-T,构建成GMCSF/IL-3融合蛋白基因,DNA序列与设计预期一致。将得到的融合蛋白基因克隆至T7RNA聚合酶表达载体pT7zz,得到表达质粒pFu,经转化至表达宿主E.coli BL21(DE3),在IPTG诱导下获得融合蛋白目的产物的直接表达。经SDS-PAGE电泳鉴定扫描分析,目的基因产物表达量占菌体总蛋白量的30%以上,目的基因表达产物以包涵体的形式表达。Westernblot鉴定表明,该表达产物可以与GM-CSF抗体及IL-3抗体特异性结合。目的基因表达产物经过包涵体变性、透析复性及柱层析纯化,用GM-CSF、IL-3依赖细胞株TF-1检测,具有明显的生物学活性。     

Prolonged Restraint Stress Increases IL-6, Reduces IL-10, and Causes Persistent Depressive-Like Behavior That Is Reversed by Recombinant IL-10

Altered inflammatory cytokine profiles are often observed in individuals suffering from major depression. Recent clinical work reports on elevated IL-6 and decreased IL-10 in depression. Elevated IL-6 has served as a consistent biomarker of depression and IL-10 is proposed to influence depressive behavior through its ability to counterbalance pro-inflammatory cytokine expression. Clinical and animal studies suggest a role for IL-10 in modifying depressive behavior. Murine restraint stress (RST) is regularly employed in the study of behavioral and biological symptoms associated with depressive disorders. While responses to acute RST exposure have been widely characterized, few studies have examined the ongoing and longitudinal effects of extended RST and fewer still have examined the lasting impact during the post-stress period. Consistent with clinical data, we report that a protocol of prolonged murine RST produced altered cytokine profiles similar to those observed in major depressive disorder. Parallel to these changes in circulating cytokines, IL-10 mRNA expression was diminished in the cortex and hippocampus throughout the stress period and following cessation of RST. Moreover, chronic RST promoted depressive-like behavior throughout the 28-day stress period and these depressive-like complications were maintained weeks after cessation of RST. Because of the correlation between IL-10 suppression and depressive behavior and because many successful antidepressant therapies yield increases in IL-10, we examined the effects of IL-10 treatment on RST-induced behavioral changes. Behavioral deficits induced by RST were reversed by exogenous administration of recombinant IL-10. This work provides one of the first reports describing the biological and behavioral impact following prolonged RST and, taken together, this study provides details on the correlation between responses to chronic RST and those seen in depressive disorders.     

重组人IL-17A和IL-17F的制备方法及活性测定

人IL-17A和IL-17F具有很高的同源性,在炎症性疾病、自身免疫性疾病和肿瘤中都发挥着重要的作用,是当前研究的热点.应用原核表达系统在大肠杆菌BL21(DE3)中高效表达了人IL-17A和IL-17F;经培养条件的优化,未发现可溶性目的蛋白的表达,免疫印记分析显示,重组蛋白位于包涵体中;对包涵体进行洗涤、凝胶过滤层析纯化和柱上复性,获得重折叠的可溶性蛋白;随后用SDS-PAGE对蛋白样品进行了纯度分析、采用免疫印记和质谱的方法鉴定蛋白产物成分、用ME3T3-E1和RAW264.7两个细胞株对IL-17A、IL-17F的生物学活性进行测定.结果显示,柱上复性的方法制备的谊重组蛋白具有较高的纯度和活性.建立的重组人IL-17A和IL-17F的制备方法可为相关研究中细胞因子的大量应用提供参考.     

In Silico Assay Development for Screening of Tetracyclic Triterpenoids as Anticancer Agents against Human Breast Cancer Cell Line MCF7

Experimental activity of a compound on cancer cell line/target is mostly analyzed in the form of percentage inhibition at different concentration gradient and time of incubation. In this study a statistical model has been developed referred as in silico assay using support vector regression model, which can act with change in concentration gradient and time of incubation. This model is a function of concentration gradient, treatment hour and independent components; which calculate the percentage inhibition in combination of above three components. This model is designed to screen tetracyclic triterpenoids active against human breast cancer cell line MCF7. The model has been statistically validated, checked for applicability domain and predicted results were reconfirmed by MTT assay, for example Oenotheranstrol derivatives, OenA & B. Computational SAR, target and docking studies were performed to understand the cytotoxic mechanism of action of Oenotheranstrol compounds. The proposed in silico assay model will work for specific chemical family for which it will be optimized. This model can be used to analyze growth kinetics pattern on different human cancer cell lines for designed compounds.     

火龙果溃疡病防治药剂的筛选

火龙果溃疡病是火龙果生产中常见的病害之一,对火龙果产量和品质的影响较大,近年来火龙果溃疡病的发生频率逐年增加.本研究通过菌丝生长抑制法测定9种杀菌剂对火龙果溃疡病病菌的杀菌活性.结果表明,戊唑·咪鲜胺、肟菌·戊唑醇、吡唑·毒氟磷有较强的抑菌作用,EC50分别为0.0209,0.0762,2.0358mg/L,本研究为生产上防治火龙果溃疡病药剂的筛选提供了参考.     

噬菌体展示重组人淋巴毒素突变体库及受体亲和筛选

淋巴毒素 (lymphotoxin , LT) 通过 TNFR1 受体传递凋亡信号,从而发挥抗肿瘤活性 . 对 LT 的受体结合区域进行多点随机突变,利用噬菌体展示重组人淋巴毒素 (rhLT) R46 , S106 , L130 三点随机突变组合文库和 S106 ～ F110 区域随机突变体库 . 噬菌体库与固相化 TNFR1 受体进行亲和筛选,富集了能与 TNFR1 受体结合的 rhLT 突变体 . 随机挑选 20 个单克隆噬菌体进行 ELISA 受体结合鉴定,其中 80 ％的克隆与 TNFR1 受体特异性结合,有 4 个克隆与 TNFR1 受体的结合能力高于野生型序列的 rhLT. 将这 4 个结合力高的突变体克隆于 pET32a(+) 载体,经过大肠杆菌表达和纯化操作后,检测这些突变体蛋白与 TNFR1 受体的结合活性和对 L929 细胞的杀伤活性,发现 3 个克隆的受体结合性质与其展示于噬菌体上时基本吻合,其中 C199 克隆与 TNFR1 的结合活性比野生型序列的 rhLT 提高了近 30 ％,且其对 L929 细胞的杀伤活性提高了近 90%. 应用噬菌体展示技术对淋巴毒素进行体外进化研究的尝试,为下一步的蛋白质结构和功能研究提供了思路,可成为大分子药物开发的有效工具 .     

Recombinant Production of Human Interleukin 6 in Escherichia coli

In this study, we compared basic expression approaches for the efficient expression of bioactive recombinant human interleukin-6 (IL6), as an example for a difficult-to-express protein. We tested these approaches in a laboratory scale in order to pioneer the commercial production of this protein in Escherichia coli (E. coli). Among the various strategies, which were tested under Research and Development (R&D) conditions, aggregation-prone IL6 was solubilized most effectively by co-expressing cytoplasmic chaperones. Expression of a Glutathion-S-Transferase (GST) fusion protein was not efficient to increase IL6 solubility. Alteration of the cultivation temperature significantly increased the solubility in both cases, whereas reduced concentrations of IPTG to induce expression of the T7lac-promotor only had a positive effect on chaperone-assisted expression. The biological activity was comparable to that of commercial IL6. Targeting the expressed protein to an oxidizing environment was not effective in the generation of soluble IL6. Taken together, the presence of chaperones and a lowered cultivation temperature seem effective to isolate large quantities of soluble IL6. This approach led to in vivo soluble, functional protein fractions and reduces purification and refolding requirements caused by downstream purification procedures. The final yield of soluble recombinant protein averaged approximately 2.6 mg IL6/liter of cell culture. These findings might be beneficial for the development of the large-scale production of IL6 under the conditions of current good manufacturing practice (cGMP).     

重组人白细胞介素15融合蛋白的表达、纯化及免疫原性检测

目的:以白细胞介素15(IL-15)为靶点,研制类风湿性关节炎免疫治疗蛋白疫苗。方法:将N端融合破伤风类毒素(TT)表位的人IL-15基因克隆至带有His标签的原核表达载体pQE-30上,转化大肠杆菌M15,经IPTG诱导表达,获得重组人TT-IL-15融合蛋白(简称rtIL-15);目的蛋白经镍柱亲和层析纯化后,用Western印迹和HPLC进行鉴定;将rtIL-15与氢氧化铝佐剂混合,免疫BALB/c小鼠,检测疫苗的免疫原性。结果:双酶切鉴定和核苷酸序列测定结果表明重组融合表达质粒pQE-30-TT-IL-15构建正确,重组蛋白的表达量达到菌体总蛋白的20%,主要以包涵体形式表达,经过纯化、复性后,目的蛋白纯度达到95%以上;蛋白疫苗免疫小鼠后,能诱导高滴度的特异性的IL-15抗体。结论:在大肠杆菌中表达了重组人IL-15融合蛋白疫苗,并具有良好的免疫原性。     

Human Recombinant B7-H3 Expressed in E.colt Enhances T Lymphocyte Proliferation and IL-10 Secretion in Vitro

Since it was proposed in 1970, the two-signal hypothesis for T lymphocyte activation became widely accepted, which elucidated T cells required two distinct signals for optimal T helper precursor cell expansion. This model hypothesized that peptides presen…     

重组人IL-18-EGF的双顺反子表达及其对NK细胞和肝癌细胞的影响

构建重组人IL-18-EGF肿瘤靶向分子双顺反子原核表达系统,研究重组人IL-18-EGF融合蛋白对人自然杀伤细胞（natural killer cell,NK细胞）和人肝癌细胞（SMMC-7721）的影响。构建重组人IL-18-EGF原核双顺反子表达系统pET28a（＋）-proIL-18-EGF-Caspase-4/BL21,重组蛋白经纯化后,作用于NK细胞,应用CCK-8法和ELISA试剂盒分别检测NK细胞的增殖情况和IFN-γ的分泌量。Cy3荧光标记IL-18-EGF检测融合蛋白与肿瘤细胞表面EGFR的结合情况。IL-18-EGF与NK细胞共同孵育24 h后,取培养上清液作用于人肝癌细胞SMMC-7721,分别使用细胞划痕实验和Transwell小室实验检测IL-18-EGF对肝癌细胞迁移和侵袭能力的影响。实验结果显示：重组人IL-18-EGF能加快NK细胞的增殖,促进NK细胞分泌IFN-γ;IL-18-EGF能与肿瘤细胞表面EGFR特异性结合;细胞划痕实验中,重组人IL-18-EGF组空白区域的抗填充能力高于对照组;Transwell小室实验中,12,24,48 h时IL-18-EGF组细胞穿膜数分别为94.6±2.9、101.8±4.0和116.2±4.5,均显著低于相应时间的对照组（分别为128.6±8.5、133.0±7.5和138.8±5.4）（P〈0.05）。以上结果表明,IL-18-EGF对人肝癌细胞SMMC-7721的迁移和侵袭能力有明显的抑制作用,能提高机体的免疫能力,有可能作为辅助药物运用于肝癌的治疗。     

表达全人源抗人IgE单抗的细胞株构建及筛选

目的:构建及筛选高效表达原创性全人源抗人Ig E单克隆抗体的重组工程细胞株。方法:将采用核糖体展示技术筛选到的原创性全人源抗人Ig E单链抗体(sc Fv)基因改构设计为Ig G1κ型全长抗体,构建重组真核表达质粒并电转染CHO-S细胞,Dot-blot法选取多株高表达克隆进行40ml摇瓶批次培养,再据细胞生长特征及抗体表达量选取高表达克隆进行40ml摇瓶及3L摇瓶流加培养研究,选取候选细胞株并对改构前后抗体的生物学活性进行比较研究。结果:成功构建了p MH3-H、p MH3-L、p CApuro-H、p CApuro-L四种重组真核表达质粒并成功共转染CHO-S细胞。完成了4次电转染8轮细胞克隆筛选,获得两株表达量较高的候选克隆Mab1#和Mab2#,在3L摇瓶流加培养中抗体表达量分别达到470mg/L及499mg/L。生物膜光干涉技术(Bio-Layer Interferometry,BLI)亲和力结果显示Mab1#及Mab2#两株单抗亲和力均达到nmol/L级(10-9),与现有唯一上市的抗人Ig E单抗药物奥马珠单抗(Omalizumab)的亲和力相当。选取Mab1#全长抗体与其改构前的母本单链抗体的表面等离子共振技术(surface plasmon resonance,SPR)中和活性比较结果显示Mab1#抑制h Ig E与FcεRI结合的EC50为3nmol/L,EC90为9nmol/L,较改造前亲和力提高了4.3倍,中和活性(EC50)提高了23.7倍,中和活性(EC90)提高了41.3倍。结论:成功将表达原创性全人源抗人Ig E的单链抗体(约25k Da)改造为亲和力及中和活性均大幅提升的全长抗体(约150k Da),获得2个候选细胞株。     

New Agents for Targeting of IL-13RA2 Expressed in Primary Human and Canine Brain Tumors

Interleukin 13 receptor alpha 2 (IL-13RA2) is over-expressed in a vast majority of human patients with high-grade astrocytomas like glioblastoma. Spontaneous astrocytomas in dogs resemble human disease and have been proposed as translational model system for investigation of novel therapeutic strategies for brain tumors. We have generated reagents for both detection and therapeutic targeting of IL-13RA2 in human and canine brain tumors. Peptides from three different regions of IL-13RA2 with 100% sequence identity between human and canine receptors were used as immunogens for generation of monoclonal antibodies. Recombinant canine mutant IL-13 (canIL-13.E13K) and canIL-13.E13K based cytotoxin were also produced. The antibodies were examined for their immunoreactivities in western blots, immunohistochemistry, immunofluorescence and cell binding assays using human and canine tumor specimen sections, tissue lysates and established cell lines; the cytotoxin was tested for specific cell killing. Several isolated MAbs were immunoreactive to IL-13RA2 in western blots of cell and tissue lysates from glioblastomas from both human and canine patients. Human and canine astrocytomas and oligodendrogliomas were also positive for IL-13RA2 to various degrees. Interestingly, both human and canine meningiomas also exhibited strong reactivity. Normal human and canine brain samples were virtually negative for IL-13RA2 using the newly generated MAbs. MAb 1E10B9 uniquely worked on tissue specimens and western blots, bound live cells and was internalized in GBM cells over-expressing IL-13RA2. The canIL-13.E13K cytotoxin was very potent and specific in killing canine GBM cell lines. Thus, we have obtained several monoclonal antibodies against IL-13RA2 cross-reacting with human and canine receptors. In addition to GBM, other brain tumors, such as high grade oligodendrogliomas, meningiomas and canine choroid plexus papillomas, appear to express the receptor at high levels and thus may be appropriate candidates for IL-13RA2-targeted imaging/therapies. Canine spontaneous primary brain tumors represent an excellent translational model for human counterparts.     

重组人白介素-12在银纹夜蛾中的表达纯化及其生物活性

KB细胞经PDBu刺激,采用异硫氰酸胍一步法提取细胞总RNA,RT-PCR法获得重组人白介素-12(rhIL-12) P35和P40 cDNA.将hIL-12 P35 cDNA和P40 cDNA分别克隆到pAcUW51载体的Polyhedrin和P10启动子下游,构建pAcUW51-IL12转移载体.pAcUW51-IL12与坏死缺陷型线性苜蓿银纹夜蛾核型多角体病毒基因DNA共转染Sf9细胞,获得重组杆状病毒Ac-hIL12.该病毒经血腔感染银纹夜蛾幼虫,采用亲和层析法纯化rhIL-12;SDS-PAGE(银染法)、Western blot鉴定表达和纯化的产物;ELISA检测rhIL-12含量;MTT法检测rhIL-12样品生物活性.rhIL-12分子量为75kD.rhIL-12在Sf9细胞培养中表达水平为17.8μg/106细胞;在银纹夜蛾幼虫中表达水平为200-300mg/L血淋巴.纯化的重组rhIL-12样品对经PHA-P激活的PBMC有明显的增殖活性,且具有明显的促NK细胞杀伤活性的生物活性.     

重组人白介素—12在银纹夜蛾中的表达纯化及其生物活性

KB细胞经PDBu刺激 ,采用异硫氰酸胍一步法提取细胞总RNA ,RT PCR法获得重组人白介素 12 (rhIL 12 )P35和P4 0cDNA。将hIL 12P35cDNA和P4 0cDNA分别克隆到 pAcUW 5 1载体的Polyhedrin和P10启动子下游 ,构建 pAcUW 5 1 IL12转移载体。pAcUW 5 1 IL12与坏死缺陷型线性苜蓿银纹夜蛾核型多角体病毒基因DNA共转染Sf9细胞 ,获得重组杆状病毒Ac hIL12。该病毒经血腔感染银纹夜蛾幼虫 ,采用亲和层析法纯化rhIL 12 ;SDS PAGE(银染法 )、Westernblot鉴定表达和纯化的产物 ;ELISA检测rhIL 12含量 ;MTT法检测rhIL 12样品生物活性。rhIL 12分子量为 75kD。rhIL 12在Sf9细胞培养中表达水平为 17.8μg/10 6细胞 ;在银纹夜蛾幼虫中表达水平为 2 0 0 - 30 0mg/L血淋巴。纯化的重组rhIL 12样品对经PHA P激活的PBMC有明显的增殖活性 ,且具有明显的促NK细胞杀伤活性的生物活性