四联鲎抗菌肽Tachyplesin Ⅱ毕赤酵母重组质粒构建及其表达

利用重组毕赤酵母表达四联鲎抗菌肽Tachyplesin Ⅱ以实现高效制备。根据鲎抗菌肽Tachyplesin Ⅱ的氨基酸序列,以及胰弹性蛋白酶和羧肽酶A的特异性裂解位点,设计四联鲎抗菌肽(4Tp Ⅱ)序列,按照毕赤酵母密码子偏好性进行优化,经EcoR Ⅰ和Not Ⅰ双酶切后构建重组质粒pPICZαA-4Tp Ⅱ,电转至毕赤酵母X-33,利用Zeocin抗性筛选阳性转化子,经甲醇诱导表达后SDS-PAGE分析。成功构建重组质粒pPICZαA-4Tp Ⅱ,并筛选出阳性转化子,经30℃、250 r/min、1%甲醇诱导表达5 d后,获得重组蛋白,可为高效制备鲎抗菌肽Tachyplesin Ⅱ奠定基础。

抗菌肽(tachyplesin Ⅰ)串联基因的构建、表达及抗菌活性

为了实现通过基因工程方法制备具有稳定结构的抗菌肽tachyplesinⅠ,采取了tachyplesinⅠ基因串联表达的方法。实验以高拷贝穿梭表达载体pSBPTQ为表达载体,通过RT-PCR扩增tachyplesinⅠ基因(tac)和采用直接退火的方法合成tachyplesinⅠ串联基因(2tac)。构建重组表达载体pSBPTQ-TAC和pSBPTQ-2TAC,转化到枯草杆菌WB800实现高效表达,经2%蔗糖诱导获得表达串联产物(2TAC)和TAC。通过离子交换柱层析纯化后得表达产物2TAC和TAC,2TAC经BrCN水解后,对表达产物抑菌活性分析,观察发酵液上清对大肠杆菌(E.coli K88)和伤寒沙门氏菌(Salmonella typhi)的抑菌圈和细胞微观形态的变化。实验结果表明:基因tac和2tac在枯草杆菌中表达成功,表达产物在发酵上清液中的含量分别约为8.25、17.36 mg L 1;表达产物TAC和2TAC对大肠杆菌K88和伤寒沙门氏菌都具有明显的抑菌作用,2TA C经BrCN水解产物抑菌活力高于TAC。

Tachyplesin-I对胃腺癌BGC-823细胞膜作用的质量浓度阈值

目的探讨抗菌肽tachyplesin-I对胃腺癌BGC-823细胞膜的作用机制。方法 BGC-823细胞用不同质量浓度tachy-plesin-I处理,再用台盼蓝拒染法测定活细胞率,荧光分光光度计检测细胞膜荧光素渗漏,激光共聚焦显微镜和电镜观察细胞膜的破坏情况。结果低质量浓度(≤25mg/L)tachyplesin-I对细胞存活没有明显影响,细胞膜荧光素渗漏较少[(15.14±0.05)～(17.84±0.68)];高质量浓度tachyplesin-I(≥50mg/L)使细胞存活率明显下降,细胞膜荧光素渗漏较多[(60.54±4.08)～(67.57±0.18)],并进一步引起细胞死亡。结论 tachyplesin-I对BGC-823细胞膜存在质量浓度阈值,低质量浓度tachyplesin-I引起膜可逆性通透,高质量浓度tachyplesin-I造成细胞膜严重损伤。

抗菌肽Tachyplesin Ⅰ及衍生物对大肠杆菌细胞膜作用机制的对比研究

本研究通过测定抗菌肽tachyplesinⅠ(TPⅠ)及其衍生肽TPⅠ-Y4对脂质体膜的作用模式,以及作用大肠杆菌后对细菌表面电位、疏水性及内、外膜渗透性和离子泄漏率的影响,对比探究了两个肽以细菌细胞膜为靶点的抑菌机理。结果表明:TPⅠ/TPⅠ-Y4作用后的大肠杆菌表面电位升高,表面疏水性增强,TPⅠ-Y4引起电位升高和疏水性增强稍高于TPⅠ。TPⅠ/TPⅠ-Y4均能在插入磷脂双分子层时扰乱脂质体膜释放出钙黄绿素,TPⅠ-Y4引起荧光素的泄漏率更高,但它并不完全破裂脂质体膜。TPⅠ/TPⅠ-Y4均能增加细菌内、外膜的通透性,相比之下,TPⅠ-Y4诱导的外膜渗透性较强,对细胞质膜的破坏作用较大,引起离子以及胞内大分子的泄漏量较多。TPⅠ-Y4对大肠杆菌细胞膜产生了更大的破坏作用可能是其抑菌活性相比于TPⅠ显著提高的主要原因。

抗菌肽TachyplesinⅠ的分子设计、结构与活性分析

本研究旨在抗菌肽TachyplesinⅠ(TPⅠ)的结构活性基础上,重新设计一种全新的抗菌肽TPⅠ-Y4。保持母肽链长与电荷数不变,将序列中形成TPⅠ两个二硫键的4个半胱氨酸用酪氨酸进行替换后得到TPⅠ-Y4。经生物信息学软件分析,与TPⅠ相比,TPⅠ-Y4的热稳定性更好,亲水性更强,同时具有与母肽相似的结构与抗菌活性。化学合成后经圆二色谱检测发现,TPⅠ-Y4在水相及在模拟细胞膜疏水环境的50%三氟乙醇中都表现出β-折叠结构,疏水环境中TPⅠ-Y4的β-折叠含量高于水相,也高于不同环境中的TPⅠ。抑菌试验表明,TPⅠ-Y4对细菌和真菌都有较强抑菌活性,且对细菌的抑菌活性强于TPⅠ。TPⅠ-Y4对小鼠红细胞溶血性降低,并保留了很强的内毒素中和能力,浓度为40μg·mL^(-1)时中和率可达50%以上。TPⅠ-Y4抗菌活性的提高以及溶血活性的降低,可能与β-折叠强形成者酪氨酸的替代有关,进而导致抗菌肽分子中β-折叠结构增强。

Effects of tachyplesin on the morphology and ultrastructure of human gastric carcinoma cell line BGC-823

AIM To investigate the morphological andultrastructural changes in the human gastriccarcinoma cell line BGC-823 after being treatedwith tachyplesin.METHODS Tachyplesin was isolated from acidextracts of Chinese horseshoe crab(Tachypleustridentatus)hemocytes.BGC-823 cells and thecells treated with 2.0mg/L tachyplesin wereexamined respectively under light microscope,scanning and transmission electron microscope.RESULTS BGC-823 cells had undergone therestorational alteration in morphology andultrastructure after tachyplesin treatment.Thechanges were as follows:the shape of cells wasunanimous,the volume enlarged and cellsturned to be flat and spread,the nucleo-cytoplasmic ratio lessened and nuclear shapebecame rather regular,the number of nucleolusreduced and its volume lessened,heter-chromatin decreased while euchromatinincreased in nucleus.In the cytoplasm,mitochondria grew in number with consistentstructure relatively,Golgi complex turned to betypical and well-developed,rough endoplasmicreticulum increased and polyribosomedecreased.The microvilli at cellular surfacewere rare and the filopodia reduced whilelamellipodia increased at the cell edge.CONCLUSION Tachyplesin could alter themalignant morphological and ultrastructuralcharacteristics of human gastric carcinoma cellseffectively and have a certain inducing differen-tiation effect on human gastric carcinoma cells.

TAT PTD-Tachyplesin融合基因的重叠延伸PCR法合成

为探讨HIV-Tat蛋白转导域(protein transduction domain,PTD)对中国鲎抗菌肽tachyplesin的协同作用,试验以经毕赤酵母密码子优化后的tachyplesin成熟肽(54 aa)加TAT PTD(11 aa)的cDNA序列为参考模板,设计了6条单链寡核苷酸片段,首尾引物的5'端分别引入EcoR I和Xba I酶切位点,通过重叠延伸PCR方法成功合成了TAT PTD+Tachyplesin序列,序列全长219 bp,为其后续功能与协同作用研究奠定了基础。

Effects of tachyplesin and n-sodium butyrate on proliferation and gene expression of human gastric adenocarcinoma cell line BGC-823

AIM： To investigate the effects of tachyplesin and n-sodium butyrate on proliferation and gene expression of human gastric adenocarcinoma cell line BGC-823. METHODS： Effects of tachyplesin and n-sodium butyrate on proliferation of BGC-823 cells were determined with trypan blue dye exclusion test and HE staining. Effects of tachyplesin and n-sodium butyrate on cell cycle were detected by flow cytometry. Protein levels of c-erbB-2, c-myc, p53 and p16 were examined by immunocytochemistry. RESULTS： The inhibiting effects were similar after 2.0 mg/L tachyplesin and 2.0 mmol/L n-sodium butyrate treatment, the inhibitory rate of cellular growth was 62.66% and 60.19% respectively, and the respective maximum mitotic index was decreased by 49.35% and 51.69% respectively. Tachyplesin and n-sodium buD/rate treatment could markedly increase the proportion of cells at G0/G1 phase and decrease the proportion at S phase. The expression levels of oncogene c-erbB-2, c-myc, and mtp53 proteins were down-regulated while the expression level of tumor suppressor gene p16 protein was up-regulated after the treatment with tachyplesin or n-sodium buD/rate. The effects of 1.0 mg/L tachyplesin in combination with 1.0 mmol/L n-sodium butyrate were obviously superior to their individual treatment in changing cell cycle distribution and expression of c-erbB-2, c-myc, mtp53 and p16 protein. The inhibitory rate of cellular growth of BGC-823 cells after combination treatment was 62.29% and the maximum mitotic index wasdecreased by 51.95%. CONCLUSION： Tachyplesin as a differentiation inducer of tumor cells has similar effects as n-sodium butyrate on proliferation of tumor cells, expression of correlative oncogene and tumor suppressor gene. It also has a synergistic effect on differentiation of tumor cells.

Effects of tachyplesin on the regulation of cell cycle in human hepatocarcinoma SMMC-7721 cells

AIM: To investigate the effects of tachyplesin on the cell cycle regulation in human hepatcarcinoma cells.METHODS: Effects of tachyplesin on the cell cycle in human hepatocarcinoma SMMC-7721 cells were assayed with flow cytometry. The protein levels of p53, p16, cyclin D1 and CDK4 were assayed by immunocytochemistry. The mRNA levels of p21WAF1/CIP1 and c-myc genes were examined with in situ hybridization assay.RESULTS: After tachyplesin treatment, the cell cycle arrested at G0/G1 phase, the protein levels of mutant p53, cyclin D1 and CDK4 and the mRNA level of c-myc gene were decreased, whereas the levels of p16 protein and p21wWF1/CIP1 mRNA increased.CONCLUSION: Tachyplesin might arrest the cell at G0/G1 phase by upregulating the levels of p16 protein and p21WAF1/CIP1 mRNA and downregulating the levels of mutant p53, cyclin D1 and CDK4 proteins and c-myc mRNA, and induce the differentiation of human hepatocacinoma cells.

Effects of tachyplesin on proliferation and differentiation of human hepatocellular carcinoma SMMC-7721 cells

AIM: To investigate the antitumor activities of tachyplesin on human hepatocellula r carcinoma (HCC) cells.METHODS: Tachyplesin, isolated from acid extracts of Chinese horseshoe crab (Tachypleus tridentatus) hemocytes, was used to treat the human HCC cell line SMMC-7721. Effects of tachyplesin on the proliferation of SMMC-7721 cells were measured with trypan blue dye exclusion test and HE staining. The morphology and ultrastructure of the cells were examined by light microscopy and transmission electron microscopy, respectively. The activities of γ-glutamyltransferase (γ-GT) and tyrosine aminotransferase (TAT) were assayed with biochemical methods. The levels of alpha fetoprotein (α-FP), proliferating cell nuclear antigen (PCNA), p21wAF1/CIP1 and c-myc were examined by immunocytochemistry. RESULTS: After treatment with tachyplesin 3.0 mg/L, the proliferation of SMMC-7721 cells was inhibited significantly, with the cell growth inhibitory rate amounted to 55.57 % and the maximum cell mitotic index declined by 43.68 %. The morphology and ultrastructure underwent restorational alteration. The activity of γ-GT declined while TAT activity increased obviously, and the levels of α-FP and PCNA decreased. Moreover, the expression of p21WAF1/CIP1 protein was upregulated and that of c-myc protein was down-regulated. CONCLUSION: Tachyplesin could effectively inhibit the proliferation of hepatocarcinoma cells, reverse the malignant morphological and ultrastructural characteristics, alter the levels of enzymes and antigens, regulate the expression of differentiation-associated oncogene and tumor suppressor gene, and induce hepatocarcinama cell differentiation.

鲎肽素(tachyplesins)、tachystatins和polyphemusins

本文介绍分离自中国鲎、美洲鲎的三个肽类物质,即鲎肽素(tachyplesin)、tachystatin、 polyphemusin及其氨基酸序列、生物活性、应用前景。

Artificial Synthesis of TAT PTD-Tachyplesin Fusion Gene by Overlap Extension PCR

This study aimed to investigate the synergism of the TAT PTD （ protein transduction domain in HIV-1 transactivator of transcription protein） to antibacte- rial peptide tachyplesin from Tachp/eus tr/dentatus. Treated with Pichia pastoris preferred codon optimization, using the eDNA sequence of tuchyplesin mature pep- tide （54 aa） harboring TAT FFD sequence （11 aa） as reference template, six single-stranded oligonueleotides were designed, the sequences of restriction sites EcoR I and Xba I were introduced to the 5＇ end of primers P1 and P6, respectively. TAT PTD ＋ Tachyplesin fusion gene with a full length of 219 bp was artificially synthesized by overlap extension PCR, which laid the preliminary foundation for subsequent functional and synergism studies.

人溶菌酶-抗菌肽tachyplesins融合蛋白的原核表达及其抗菌活性

目的原核表达人溶菌酶(Human lysozyme,hLYZ)和抗菌肽tachyplesins融合蛋白,并检测其抗菌活性。方法人工合成抗菌肽tachyplesins基因和linker,与pMD18-T-hLYZ上切下的hLYZ基因融合,将融合基因克隆至带有GST标签的原核表达载体pGEX-4T-1上,转化大肠杆菌BL21(DE3),IPTG诱导表达,并对表达条件进行优化。表达的融合蛋白经亲和层析纯化后,进行抗菌活性检测。结果重组表达质粒pGEX-4T-1-hLYZ-tachyplesins经PCR、双酶切及测序鉴定,证明构建正确;表达产物经SDS-PAGE分析,在相对分子质量约44000处可见目的蛋白条带,诱导温度在25℃,IPTG终浓度为0.8mmol/L,诱导时间为6h,融合蛋白表达效果较好,主要以可溶性形式存在;纯化的融合蛋白纯度可达90%以上,对金黄葡萄球菌和大肠杆菌具有一定的抑制作用。结论已成功在原核细胞中表达了人溶菌酶-抗菌肽tachyplesins融合蛋白,纯化的融合蛋白具有一定的抗菌活性。

合成抗菌肽TachyplesinⅠ的体外生物活性及其降解规律

目的探讨合成抗菌肽TachyplesinⅠ在体外的生物活性及在模拟消化环境中的降解规律。方法采用不同温度、pH值、阳离子浓度、溶剂极性、模拟消化环境分别处理TachyplesinⅠ,通过检测TachyplesinⅠ生物活性的变化分析其稳定性;检测TachyplesinⅠ对小鼠血细胞的溶血活性;通过HPLC图谱变化评定TachyplesinⅠ在模拟消化环境中的降解情况。结果 TachyplesinⅠ在低于100℃、pH值小于10.3的情况下具有稳定性,阳离子浓度和溶液极性对TachyplesinⅠ的抗菌活性具有一定影响;在TachyplesinⅠ浓度大于80 mg/L时,作用时间大于30 min时,表现出一定的溶血活性;TachyplesinⅠ在模拟胃液、胃黏膜匀浆和血浆系统中表现出很高的稳定性,色谱峰型基本未改变,几乎无降解作用,TachyplesinⅠ的最小抑菌浓度为5.0～20.0 mg/L;在模拟小肠液和小肠黏膜匀浆系统中稍微敏感,色谱峰型降低,出现小杂峰,生物活性明显降低,最小抑菌浓度在80～160 mg/L之间。结论 TachyplesinⅠ具有较强的高温耐受性,在酸性条件下稳定,同时具有一定的耐受体内蛋白酶降解的能力。

Expression of tachyplesin gene in yeast Pichia pastoris

Tachyplesin gene was designed and chemically synthesized with codon usage bias. The stop codon TAG and some restriction sites convenient for further cloning were added to this gene. The synthesized gene cloned into yeast expression vector pPIC9 (with α_secretion signal) was transformed into host strain GS115 by electroporation. The tachyplesin expressed from recombinants Y PIC27 and Y PIC42 showed an inhibition activity against the germination of the spores of \%Magnaporthe grisea\%. Southern blot performed with chromosome genome of the two recombinants indicated a single copy of the expression cassette was integrated at the chromosomal AOX 1 locus by which the genomic AOX 1 gene was functionally disrupted and Northern blot showed the presence of transcripts of the tachyplesin gene.

海洋生物抗菌肽在枯草杆菌BS168中的高效表达

为了实现基因工程高效制备tachyplesin Ⅰ,采用tachyplesin Ⅰ基因串联表达的方法,以穿梭表达载体pSBPTQ为表达载体,通过RT-PCR扩增tachyplesinⅠ基因(tac)和采用直接退火的方法合成tachyplesinⅠ串联基因(2tac),构建重组表达载体pSBPTQ-TAC和pSBPTQ-2TAC,转化到枯草杆菌BS168实现高效表达。实验结果表明:基因tac和2tac在枯草杆菌中表达成功,TAC和2TAC抗菌肽表达量分别约为8.5%、15.8%,经高效液相色谱分析表达产物在发酵上清液中的含量约为5.46、10.36 mg/L;表达产物TAC和2TAC对大肠杆菌K88和金黄色葡萄球菌都具有明显的抑菌作用,2TAC经BrCN水解产物抑菌活力高于TAC,而2TAC的表达产量大约是TAC的1.89倍。这表明通过tachyplesin Ⅰ串联表达产物降低了自身对宿主的毒性,可以提高tachyplesin Ⅰ的表达产量。

中国鲎鲎素诱导人肝癌SMMC-7721细胞分化的观察

背景与目的:海洋生物活性物质抗肿瘤活性研究是海洋生物活性物质开发与抗癌药物研究的一个重要领域。诱导肿瘤细胞分化则是肿瘤药物治疗的新策略。本文拟研究海洋生物活性物质鲎素对人肝癌SMMC-7721细胞分化的影响,以为鲎素抗肿瘤作用及其机理的深入研究提供实验依据。方法:从中国鲎血细胞酸抽提液提取鲎素,应用光镜和透射电镜观察3.0μg/ml鲎素处理前后人肝癌SMMC-7721细胞形态和超微结构的变化,应用细胞化学或免疫细胞化学方法观察鲎素处理前后细胞碱性磷酸酶活性与甲胎蛋白和增殖细胞核抗原表达的变化。结果:经3.0μg/ml鲎素处理的SMMC-7721细胞形态和超微结构发生恢复性变化,碱性磷酸酶活性减弱,甲胎蛋白和增殖细胞核抗原表达降低。结论:鲎素能有效改变肝癌细胞恶性形态和超微结构特征,改变肝癌细胞相关酶活性和抗原表达,对肝癌细胞具有一定的诱导分化作用。

中国鲎鲎素对人胃癌BGC-823细胞增殖的抑制作用

应用从中国鲎血细胞中提取的鲎素处理人胃癌 BGC- 82 3细胞 ,研究海洋生物活性物质的抗肿瘤作用 .实验结果显示 ,经 2 .0 μg/m L鲎素处理的 BGC- 82 3细胞生长缓慢 ,倍增时间延长 ,细胞集落形成能力减弱 ,细胞生长抑制率达 62 .67% ,细胞分裂指数下降 4 0 .91% .处理后细胞碱性磷酸酶细胞化学反应减弱、分布改变 ,碱性磷酸酶和乳酸脱氢酶活力分别下降 4 0 .59%和 76.0 5% .结果表明 ,鲎素能有效地抑制胃癌细胞的增殖活动 ,具有与癌细胞诱导分化物相似的抗肿瘤效果 .

鲎素抗菌肽的分子结构稳定性及生物活性

为了实现鲎素这种高效、广谱的抗菌肽在生产实践中的应用,采用不同温度、pH值、体外蛋白酶（胃蛋白酶、胰蛋白酶、弹性蛋白酶、羧肽酶B）分别处理鲎素,通过检测鲎素最小抑菌浓度（M IC）的变化来衡量鲎素的生物活性稳定性;采用高效液相色谱（HPLC）检测鲎素残留量,通过HPLC图谱变化来评定鲎素分子结构的稳定性.结果表明：温度小于120℃、pH值小于11.30时,鲎素对大肠杆菌K88的M IC为1.25～5.00mg/L;高效液相色谱检测得鲎素残留量在65.46～70.21μg之间;鲎素对胃蛋白酶的作用表现出很高的稳定性,对胰蛋白酶、羧肽酶B、弹性蛋白酶的作用稍微敏感;在胃蛋白酶酶活浓度不高于5.33mmol/（s.L）、胰蛋白酶酶活浓度不高于0.67mmol/（s.L）、羧肽酶B酶活浓度不高于0.17mmol/（s.L）、弹性蛋白酶酶活浓度不高于0.021mmol/（s.L）的条件下,鲎素仍具有活性.这说明鲎素抗菌肽具有较强的高温耐受性,在酸性条件下具有稳定性,且具有一定的耐受蛋白酶降解的能力.

鲎素的抗菌靶点初探

采用体外抑菌法测定鲎素的抑菌动力学特点,钼酸铵比色法和紫外吸收法分别检测细菌与鲎素共同孵育前后无机磷和大分子泄漏情况,扫描电镜和透射电镜观察细菌与鲎素共同孵育前后细菌形态和结构的变化,紫外吸收法和凝胶电泳法分别观察鲎素对细菌基因组DNA和质粒DNA结构的影响,质粒转化实验检测鲎素对质粒DNA复制和转录功能的影响.结果表明,鲎素对革兰氏阳性菌和阴性菌具有不同的抑菌动力学特点,经鲎素处理的细菌,胞内无机磷和大分子泄漏显著,细胞壁膜和菌体遭到不同程度的破坏,鲎素可与细菌基因组DNA和质粒DNA结合,高浓度鲎素有可能使DNA发生断裂,进而使质粒DNA复制和转录功能受到抑制.上述结果提示,鲎素的抗菌靶点至少包括细胞壁膜和菌体DNA.