Doublecortin-like kinase 1在消化系统肿瘤中的表达及意义

随着人们对于消化道肿瘤的研究逐渐深入,诊断方法和治疗手段需要更加直接和准确。寻找可靠的肿瘤干细胞标志物一直是肿瘤研究中的重点。Doublecortin-like kinase 1(DCLK1)是近些年发现的可能的癌干细胞标志物之一,在多种恶性肿瘤组织中表达,如结直肠癌、胰腺肿瘤、前列腺癌、肝细胞癌等,并且在肿瘤的发展过程中起到功能性作用。本文综述DCLK1的结构及其在消化系统肿瘤中表达意义的相关文献,为DCLK1的有关研究和新型抗癌靶向药物研制提供参考。

Doublecortin-like kinase 1 exhibits cancer stem cell-like characteristics in a human colon cancer cell line

Objective： Colon cancer stem cells （CSCs） are implicated in colorectal cancer carcinogenesis, metastasis, and therapeutic resistance. The identification of these cells could help to develop novel therapeutic strategies. Doublecortin-like kinase 1 （DCLK1） has been viewed as a marker for gastrointestinal stem cells that fuel the self-renewal process, however others view them as a marker of Tuft cells or as an enteroendocrine subtype. The purpose of this study was to use a colon cancer cell line to identify and characterize the stem-like characteristics of the DCLKI＋ cell population. Methods： To enrich stem-like cells, HCT116 cells （derived from colon adenocarcinomas） were cultured using serum-free media to form spheres under both normal oxygen and hypoxia condition. DCLK1 transcript expression in the adherent parental cells and spheroids was quantified using quantitative real time reverse transcription- polymerase chain reaction [（q）RT-PCR]. DCLK1 protein expression was determined using flow cytometry. Self-renewal capability from adherent parental cells and spheroids was determined using extreme limiting dilution analysis （ELDA）. Results： Under both normal oxygen and hypoxia condition, the adherent parental cells were composed of cells that express low levels of DCLK1. However, spheroids exhibited an increased frequency of cells expressing DCLK1 on both mRNA and protein levels. Cells derived from spheroids also possess stronger self-renewal capability. Conclusions： The higher fraction of DCLK1 ＋ cells exhibited by spheroids and hypoxia reflects the stem- like characteristics of these cells. DCLK1 may represent an ideal marker to study and develop effective strategies to overcome chemo-resistance and relapse of colon cancer.

Role of doublecortin-like kinase 1 and leucine-rich repeat-containing G-protein-coupled receptor 5 in patients with stage Ⅱ/Ⅲ colorectal cancer:Cancer progression and prognosis

BACKGROUND Cancer stem cells(CSCs)are a subpopulation of cancer cells with the potential of self-renewal and differentiation.CSCs play critical roles in tumorigenesis,recurrence,metastasis,radiation tolerance and chemoresistance.AIM To assess the expression patterns and clinical potential of doublecortin-like kinase 1(DCLK1)and leucine-rich repeat-containing G-protein-coupled receptor 5(Lgr5),as prognostic CSC markers of colorectal cancer(CRC).METHODS The expression of DCLK1 and Lgr5 in CRC tissue sections from 92 patients was determined by immunohistochemistry.Each case was evaluated using a combined scoring method based on signal intensity staining(scored 0-3)and the proportion of positively stained cancer cells(scored 0-3).The final staining score was calculated as the intensity score multiplied by the proportion score.Low expression of DCLK1 and Lgr5 was defined as a score of 0-3;high expression of DCLK1 and Lgr5 was defined as a score of≥4.Specimens were categorized as either high or low expression,and the correlation between the expression of DCLK1 or Lgr5 and clinicopathological factors was investigated.RESULTS DCLK1 and Lgr5 expression levels were significantly positively correlated.CRC patients with high DCLK1,Lgr5 and DCLK1/Lgr5 expressions had poorer progression-free survival and overall survival.Moreover,high expression of DCLK1 was an independent prognostic factor for recurrence and overall survival in patients with CRC by multivariate analysis(P=0.026 and P=0.049,respectively).CONCLUSION DCLK1 may be a potential CSC marker for the recurrence and survival of CRC patients.

RNAi沉默Polo-like kinase-1基因表达对大肠癌细胞端粒酶活性的影响

目的探讨polo-like kinase-1(PLK1)基因对大肠癌细胞增殖和端粒酶活性的影响。方法根据PLK1基因序列特点,设计并用化学方法合成小干扰核糖核酸分子(small interfering RNA,si RNA),转染人大肠癌SW480细胞后,分别采用实时定量PCR和Western blot检测PLK1基因mRNA和蛋白表达水平。分别采用MTT法和TRAP-ELISA方法检测PLK1基因转染对大肠癌细胞增殖和端粒酶活性的影响。结果所设计的5个si RNA均能明显抑制大肠癌SW480细胞PLK1 mRNA水平,以P4效果最好。以P4转染处理大肠癌细胞后,PLK1 mRNA水平和蛋白水平明显下调,且呈浓度和时间依赖性。MTT和TRAP-ELISA方法检测发现,P4si RNA转染组细胞增殖和端粒酶活性明显受到抑制,且呈浓度和时间依赖性(P<0.05,P<0.05)。结论PLK1基因对大肠癌细胞增殖具有重要的调控作用;以PLK1 si RNA转染处理大肠癌细胞,可明显抑制大肠癌细胞的恶性增殖,其机制可能与抑制端粒酶活性有关。

EFFECT OF ACTIVE COMPOUNDS ISOLATED FROM PTERIS SEMIPINNATA L ON DNA TOPOISOMERASES AND TYROSINE PROTEIN KINASE AND EXPRESSION OF C-MYC IN LUNG ADENOCARCINOMA CELLS

Objective: To study the effect of active compound 6F and A from Pteris semipinnata L.(PsL) on the activities of DNA topoisomerase (TOPO) I and II, activities of cytosolic and membrane TPK, and expression of oncogene c-myc in lung adenocarcinoma cells. Methods: The effect of compound 6F and A on activities of cytosolic and membrane TPK was measured by scintillation counting; the effect of compound A on expression of oncogene c-myc was determined by flow cytometry indirect fluorimetry. Results: compound 6F and A could inhibit the activities of TOPO I, and they strongly inhibited the TOPO II in 0.01 mg/L and 10.0 mg/L respectively. Compound A slightly inhibited the activities of membrane TPK, but not the cytosolic one. Compound A could inhibit the expression of oncogene c-myc. Conclusion: Topoisomerases are target of compound 6F and A. Compound A could slightly inhibit the activities of TPK, and showed an inhibitory effect on the expression of oncogene c-myc.

Increased L-arginine Production by Site-directed Mutagenesis of N-acetyl-L-glutamate Kinase and pro B Gene Deletion in Corynebacterium crenatum

Objective In Corynebacterium crenatum,the adjacent D311 and D312 of N-acetyl-L-glutamate kinase(NAGK),as a key rate-limiting enzyme of L-arginine biosynthesis under substrate regulatory control by arginine,were initially replaced with two arginine residues to investigate the L-arginine feedback inhibition for NAGK.Methods NAGK enzyme expression was evaluated using a plasmid-based method.Homologous recombination was employed to eliminate the pro B.Results The IC50 and enzyme activity of NAGK M4,in which the D311 R and D312 R amino acid substitutions were combined with the previously reported E19 R and H26 E substitutions,were 3.7-fold and 14.6% higher,respectively,than those of the wild-type NAGK.NAGK M4 was successfully introduced into the C.crenatum MT genome without any genetic markers;the L-arginine yield of C.crenatum MT-M4 was 26.2% higher than that of C.crenatum MT.To further improve upon the L-arginine yield,we constructed the mutant C.crenatum MT-M4 ?pro B.The optimum concentration of L-proline was also investigated in order to determine its contribution to L-arginine yield.After L-proline was added to the medium at 10 mmol/L,the L-arginine yield reached 16.5 g/L after 108 h of shake-flask fermentation,approximately 70.1% higher than the yield attained using C.crenatum MT.Conclusion Feedback inhibition of L-arginine on NAGK in C.crenatum is clearly alleviated by the M4 mutation of NAGK,and deletion of the pro B in C.crenatum from MT to M4 results in a significant increase in arginine production.

Effects of tyrosine kinase inhibitor E7080 and eNOS inhibitor L-NIO on colorectal cancer alone and in combination

Objective：To investigate the effects of E7080 and N5-（1-iminoethyl）-L-ornithine dihydrochloride （L-NIO）on colorectal cancer alone and in combination.Methods：HT29 colorectal cancer cell line from Sap Institute was used.Real-time cell analysis （xCELLigence system） was performed to determine the effects of E7080 and L-NIO on colorectal cell proliferation.While apoptosis was determined with Annexin V staining,and the effect of agents on angiogenesis was determined with chorioallantoic membrane （CAM） model.Results：We found that E7080 has a strong antiproliferative effect with an half maximum inhibition of concentration （IC50） value of 5.60×10-8 mol/L.Also it has been observed that E7080 showed antiangiogenic and apoptotic effects on HT29 colorectal cancer cells.Antiangiogenic scores of E7080 were 1.2,t.0 and 0.6 for 100,10 and 1 nmol/L E7080 concentrations,respectively.Furthermore,apoptosis has been detected in 71％ of HT29 colorectal cancer cells after administration of 100 nmol/L E7080 which may indicate strong apoptotic effect.Meanwhile administration of L-NIO alone did not show any effect,but the combination of E7080 with L-NIO increased the antiproliferative,antiangiogenic and apoptotic effects of E7080.Conclusions：Results of this study indicate that E7080 may be a good choice in treatment of colorectal tumors.Furthermore the increased effects of E7080 when combined with L-NIO raise the possibility to use a lower dose of E7080 and therefore avoid/minimize the side effects observed with E7080.

Expression and functional analyses of the mitogen-activated protein kinase (MPK) cascade genes in response to phytohormones in wheat ( Triticum aestivum L.)

Mitogen-activated protein kinase （MPK） cascades consist of a set of kinase types （MPKKKs, MPKKs, MPKs） to establish conserved signal-transducing modules mediating plant growth, development as well as responses to internal and external cues. In this study, the expression patterns of six MPKKK, two MPKK, and 11 MPK genes in wheat in responses to external treatments of phytohormones, including naphthylacetic acid （NAA）, abscisic acid （ABA）, 6-benzyladenine （6-BA）, gibber- ellin （GA3）, salisylic acid （SA）, jasmonic acid （JA）, and ethylene （ETH）, were investigated. Expression analysis revealed that several of the MPK cascade genes are responses to the external phytohormone signaling. Of which, TaMPKKKA;3 is induced by 6-BA and NAA while TaMPK4 repressed by ETH, GA3, SA, and JA; TaMPKKKA, TaMPKKKA;3 and TaMPK1 are down-regulated by ETH and GA3whereas TaMPK9 and TaMPK12 repressed by ETH and JA in addition that TaMPK12 also repressed by GA3; TaMPK12;1 is down-regulated by ABA, GA3 and SA while TaMPK17 repressed by all exogenous phytonormones examined. TaMPK4, a MPK type gene previously characterized to mediate tolerance to phosphate （Pi） deprivation, was functionally evaluated for its role in mediation of responses of plants to exogenous GA3, ETH, SA, and JA. Results indicated that overexpression and antisense expression of TaMPK4 in tobacco dramatically modify the growth of seedlings upon treatments of GA3, SA and JA, in which the overexpressors behaved deteriorated growth feature whereas the seedlings with antisense expression of TaMPK4 exhibited improved seedling phenotype. The growth behaviors in lines overexpressing or antisensely expressing TaMPK4 are closely associated with the biomass and the corresponding hormone-associated parameters. These results demonstrated that TaMPK4 acts as a critical player in mediating the phyto- hormone signaling. Our findings have identified the phytohormone-responsive MPK cascade genes in wheat and provided a connection between the phytohormone-mediated responses and the MPK cascade pathways.

Genome-Wide Analysis of HAESA/HAESA-Like Kinase Family in Rice

In leucine-rich repeat (LRR) receptor-like kinase XI subfamily, Arabidopsis HAESA (AtHAE) and two closely related HAESA-LIKE (AtHSL1 and AtHSL2) constitute a small branch. Several reports have described the function and the involved signaling pathway that AtHAE and AtHSLs are involved in. However, the family members and functions of HAE and HSL in rice have not been reported. Here, we performed a genome-wide analysis of the HAE/HSL kinase family in rice. A total of 17 OsHSLs were identified in the genome. Of these, only Os11g11890 was annotated as HSL2;all the other members were annotated as HSL1. Phylogenetic analysis revealed that OsHSLs diverged into three groups, with three Arabidopsis members constituting a subgroup of group I. Domain analysis revealed that all the homologues had 9-19 LRR repeats and a typical kinase domain at the C-terminus, except that four members lost or evolved their kinase domains. Expression analysis revealed that OsHSLs were co-expressed with genes involved in biotic and abiotic stresses. Microarray data revealed that most OsHSLs were highly expressed in the vegetative tissues and only two members were highly expressed in the reproductive tissues. Most OsHSLs changed their expression profiles when subjected to drought, and salt stress treatments. Our results provide an overview of OsHSL gene family in rice, and suggest that OsHSLs possibly function under biotic and abiotic stresses, thus would help for elucidating the function of OsHSLs gene family in vivo.

辣椒中L型凝集素类受体激酶CaLecRKs鉴定及其对辣椒疫霉的响应

L型凝集素类受体激酶(LecRKs)广泛参与植物的先天免疫过程。目前未见在辣椒Capsicum annuum中全基因组鉴定LecRKs的报道。本研究对辣椒中的CaLecRK进行了全基因组鉴定,并在接种辣椒疫霉Phytophthora capsici条件下通过基因表达分析探究其对辣椒疫霉的响应情况,旨在挖掘参与辣椒抗疫病防御反应的CaLecRK基因。研究结果表明,辣椒基因组中共鉴定出24个CaLecRK,以其构建系统发育树发现,可将24个CaLecRK分为7个分支。基因表达分析结果显示,有4个CaLecRK基因(CaLecRK 2.2、CaLecRK 3.2、CaLecRK 8.1和CaLecRK 10.1)受辣椒疫霉诱导,和接菌后0 h相比,接菌处理后12 h或36 h基因表达差异显著,推测其在辣椒抗疫病防御反应中发挥了重要作用。

微小RNA-26b-5p对缺血性心律失常大鼠心房肌细胞L型钙通道的影响

目的探讨微小RNA(miR)-26b-5p对磷脂酰肌醇3-激酶(PI3K)/磷脂酰肌醇3,4,5-三磷酸(PIP3)信号通路的调控作用以及对缺血性心律失常大鼠心房肌细胞L型钙通道的影响。方法选择SD大鼠72只,按照随机数表法分为假手术组、模型组、LY294002组、阴性对照组、过表达组、联合组,每组12只。各组给予相应干预24h,除假手术组外的其余各组大鼠建立缺血性心律失常模型,假手术组大鼠仅开胸不结扎。建模过程中检测各组大鼠心律失常指标,采用Curtis-Walker评分法进行心律失常评分;荧光定量PCR法检测心房肌细胞中miR-26b-5p表达;全细胞膜片钳技术记录心房肌细胞L型钙通道电流(ICa-L);蛋白印迹法检测L型钙通道α1C亚基(CACNA1C)、钙调蛋白及PI3K/PIP3通路相关蛋白表达。结果与模型组比较,LY294002组大鼠左心室室性期前收缩次数、室性心动过速持续时间、心室颤动持续时间、心律失常评分、心房肌细胞ICa-L峰值密度绝对值、CACNA1C、钙调蛋白表达显著升高,磷酸化PI3K、PIP3、磷酸化蛋白激酶B(Akt)表达显著降低,过表达组大鼠左心室室性期前收缩次数、室性心动过速持续时间、心室颤动持续时间、心律失常评分、心房肌细胞ICa-L峰值密度绝对值、CACNA1C、钙调蛋白表达显著降低,miR-26b-5p、磷酸化PI3K、PIP3、磷酸化Akt表达显著升高(P<0.05)。与过表达组比较,联合组大鼠左心室室性期前收缩次数、室性心动过速持续时间、心室颤动持续时间、心律失常评分、心房肌细胞ICa-L峰值密度绝对值、CACNA1C、钙调蛋白表达显著升高,磷酸化PI3K、PIP3、磷酸化Akt表达显著降低(0.82±0.08vs1.09±0.11,0.91±0.09vs1.17±0.11,0.94±0.09vs1.20±0.12,P<0.05)。结论miR-26b-5p过表达可能通过激活PI3K/PIP3相关信号通路,阻滞缺血性心律失常大鼠心房肌细胞L型钙通道,改善心律失常表现。

利用蛋白支架复合物提高大肠杆菌MG1655的L-苹果酸产量

构建RIAD-RIDD人工蛋白支架并验证其对蛋白的共定位能力,在此基础上,利用蛋白支架对L-苹果酸生成途径关键酶Pykf和maeB进行共定位,通过形成蛋白支架复合物来促进苹果酸酶的逆向催化,从而提高大肠杆菌MG1655发酵时的L-苹果酸产量。检测结果表明,人工蛋白支架RIAD-RIDD在胞外、胞内均可有效实现蛋白共定位,在导入蛋白支架复合物后,重组大肠杆菌MG1655发酵时的L-苹果酸产量大幅提高。

素馨花水提物及其主要成分对3T3-L1细胞成脂分化的影响

该研究探讨素馨花水提物(WE)及其化学成分在3T3-L1前脂肪细胞上的降脂作用。通过将3T3-L1细胞诱导为成熟脂肪细胞,油红O染色定量和检测甘油三酯(TG)含量判断素馨花样品对脂滴的抑制作用;液质联用仪分析WE中化学成分;MTT检测素馨花及其成分对3T3-L1细胞增殖的影响;Western Blot检测AMPK、C/EBPα、FAS、ACC、CPT1、Bax、Bcl-2等蛋白表达。结果发现,WE能剂量依赖性抑制脂滴形成,其中高浓度WE(500μg/mL)能降低中性脂质含量23.59%,降低TG含量30.20%,在脂肪积累早期作用最显著,并证明其活性成分主要是橄榄苦苷,含量为13.77%。WE及橄榄苦苷能激活AMPK(123.19%和115.98%)和其下游靶点ACC(451.06%和1050.0%)的磷酸化、下调其下游靶点FAS(81.72%和60.50%)的蛋白表达,减少脂肪形成,提高CPT1(164.84%和292.19%)蛋白的表达,加快脂肪酸氧化;抑制C/EBPα(68.97%和34.57%)的表达,影响3T3-L1细胞分化;上调Bax(154.60%和139.37%)、下调Bcl-2(41.10%和45.62%)蛋白的表达,诱导脂肪细胞凋亡。结果提示,WE能在3T3-L1细胞分化过程早期抑制细胞生长、分化和脂肪合成并促进脂肪酸氧化从而有效抑制脂质积累,机制上可能通过调控AMPK和Bax/Bcl-2通路。

火炭母通过调控TLR4-TBK1信号通路改善鼠伤寒沙门菌感染小鼠空肠的炎症反应

为了探讨火炭母对鼠伤寒沙门菌感染小鼠空肠的免疫保护作用及其潜在机制。本试验将48只雌性BALB/c小鼠随机分为6个组:空白对照组、模型组、阳性药物组和火炭母高、中、低剂量组,每组8只。阳性药物组小鼠灌胃庆大霉素[20 mg/(kg·bw)],火炭母高、中、低剂量组小鼠分别按16、8和4 g/(kg·bw)剂量灌胃火炭母,空白对照组和模型组小鼠给予等体积的灭菌生理盐水,共连续给药8 d。预防性给药2 d后,每只小鼠(空白对照组除外)灌胃0.2 mL半数致死量(LD 50)鼠伤寒沙门菌(5×10^(4) CFU/mL)致病。给药结束后,处死小鼠取空肠用于组织病理学检查和Western blot。结果显示,鼠伤寒沙门菌感染后,小鼠空肠杯状细胞和肠腺红细胞增多、肠绒毛结构松散,火炭母各剂量组小鼠空肠杯状细胞和肠腺红细胞明显减少,火炭母减轻了小鼠空肠组织损伤。Western blot结果显示,与空白对照组相比,模型组小鼠空肠中免疫因子β干扰素(IFN-β)蛋白表达显著上升(P<0.05),γ干扰素(IFN-γ)蛋白表达显著下降(P<0.05),干扰素调节因子3(IRF3)、磷酸化TANK结合激酶1(p-TBK1)和Toll样受体4(TLR4)蛋白表达显著上调(P<0.05),炎性因子白介素-6(IL-6)、白介素-1β(IL-1β)和核因子κB p65(NF-κB p65)蛋白表达显著上升(P<0.05);与模型组相比,不同剂量火炭母可以不同程度降低炎症因子IL-6(P<0.05或P>0.05)、IL-1β(P<0.05)和NF-κB p65(P<0.05)蛋白表达,显著提高TLR4、β干扰素TIR结构域衔接蛋白(TRIF)蛋白的表达和TANK结合激酶1(TBK1)蛋白表达及其磷酸化水平(P<0.05),提高下游信号IRF3蛋白的表达(P<0.05)及其磷酸化水平(P<0.05或P>0.05),进而提高空肠中IFN-β(P<0.05或P>0.05)和IFN-γ(P<0.05)蛋白的表达。结果表明,火炭母通过调控TLR4-TBK1信号通路改善鼠伤寒沙门菌感染小鼠空肠的炎症反应。

百脉根不定根发育相关基因LcC2DP1的克隆与功能初步分析

为研究百脉根(Lotus corniculatus L.)C2钙依赖蛋白激酶基因LcC2DP1在不定根形成过程中的功能,通过RACE法从百脉根中克隆LcC2DP1基因,利用qRT-PCR检测其时空表达模式,并通过农杆菌介导的瞬时表达系统在百脉根中过量表达LcC2DP1并鉴定其功能。结果显示:LcC2DP1基因全长705 bp,编码235个氨基酸,分子质量为25.95 ku,与蒺藜苜蓿同源性最高(82%);在百脉根不定根分化过程中持续表达,表达部位为根、茎和叶片;与野生型亲本(WT)相比,转LcC2DP1基因百脉根(TP)的不定根分化提前1~2 d;在不定根分化的9~15 d,其总根长分别是WT的168%、155%,根体积分别是WT的249%、161%,根尖数分别是WT的156%、137%。TP百脉根的总根长(P<0.01)、根体积(P<0.01)和根尖数(P<0.05)表现出一定的发育优势,表明LcC2DP1基因可能与百脉根不定根发育调控相关。

糖尿病性心肌病患者血清PDK4,DECR1和MMP1表达水平及临床价值研究

目的探讨血清丙酮酸脱氢酶激酶同工酶4(pyruvate dehydrogenase kinase isoenzyme 4,PDK4),2,4-二烯酰辅酶A还原酶1(2,4-dienoyl coenzyme A reductase 1,DECR1)及基质金属蛋白酶1(matrix metalloproteinase 1,MMP1)的联合检测在糖尿病性心肌病(diabetic cardiomyopathy,DCM)诊断、临床分级和病情预后中的应用价值。方法选取2021年10月~2023年10月陕西省人民医院收治的126例糖尿病性心肌病(DCM组)患者及120例单纯糖尿病非心肌病患者(对照组),采用酶联免疫吸附法(ELISA)测定血清中PDK4,DECR1及MMP1蛋白表达水平,评估这三个检测指标在DCM中的诊断、临床分级和病情预后中的应用价值。结果DCM组患者血清PDK4(131.38±10.20 pg/ml),DECR1(152.06±12.57 pg/ml)及MMP1(40.27±4.02μg/ml)蛋白表达水平与对照组(82.69±8.17 pg/ml,86.14±9.55 pg/ml,17.77±0.98μg/ml)相比均明显升高,差异具有统计学意义(t=36.24,47.63,12.29,均P<0.001)。DCM组患者血清PDK4,DECR1及MMP1蛋白表达水平与NYHA心功能分级相关,随等级升高其蛋白表达水平均明显升高,差异具有统计学意义(F=24.12,30.04,12.66,均P<0.001);DCM组中重度组患者与轻度组患者比较,血清PDK4(164.92±1.35pg/ml vs 122.48±8.78pg/ml),DECR1(192.17±9.11pg/ml vs124.36±10.83pg/ml)及MMP1(84.44±7.38μg/ml vs 39.41±3.05μg/ml)蛋白表达水平均显著增高,差异具有统计学意义(t=26.33,47.12,15.41,均P<0.001)。血清PDK4,DECR1及MMP1三项联合检测DCM准确度(χ^(2)=18.23,21.37,22.07)、特异度(χ^(2)=9.72,13.43,15.12)、灵敏度(χ^(2)=12.07,16.07,17.55)与单项检测对比均明显升高,差异具有统计学意义(均P<0.05),且ROC曲线分析结果显示联合检测的AUC高达0.955,明显高于单项检测(Z=16.67,17.09,20.44,均P<0.05)。结论血清PDK4,DECR1及MMP1与DCM诊断、临床分级及病情预后有一定关联,三者联合检测有助于DCM的鉴别诊断。

乳糖发酵短杆菌lysC突变对L-赖氨酸积累的影响

从一株乳糖发酵短杆菌L-异亮氨酸生产菌中克隆出天冬氨酸激酶AK-1的编码基因ly-sC1,经DNA测序并与来自谷氨酸棒杆菌ATCC13032的野生型lysC比对发现其中有2个核苷酸1186G和1187C缺失,造成翻译提前终止。AK-1还有下列2个有效突变位点:Ala 279 Thr和Ser317 Ala。lysC1在大肠杆菌BL21中的诱导表达量约为lysC的1/4,其表观比酶活也较低,但对L-苏氨酸和L-赖氨酸协同反馈抑制不敏感。用大肠杆菌-黄色短杆菌穿梭表达载体pDXW-8将ly-sC1在野生型乳糖发酵短杆菌ATCC13869中诱导型表达,经摇瓶发酵积累L-赖氨酸7.4 g/L,在3 L发酵罐上达40 g/L。

番茄SlMAPK9-2基因分离及表达分析

促分裂原活化蛋白激酶(MAPK)信号途径在植物生长发育以及多种逆境胁迫响应和激素调控过程中发挥着至关重要的作用。为了研究MAPK基因的结构和功能,利用生物信息学分析以及PCR扩增方法从番茄中分离了1个新的MAPK基因,克隆其c DNA全长序列,命名为Sl MAPK9-2;利用NCBI数据库Blast P工具和在线软件MEME分析发现其具有MAPK保守的结构域和保守基序。系统进化树分析显示Sl MAPK9-2属于D组MAPK,与茄科植物马铃薯和烟草MAPK9位于同一进化树分支。利用数据库PGDD分析发现,Sl MAPK9-2与Sl MAPK16以及Pm MAPK9之间发生了大片段复制事件,且2个基因对的Ka/Ks均小于1,说明经历了达尔文纯化选择。实时荧光定量PCR分析发现,Sl MAPK9-2在不同组织器官中均有表达,在开放花中表达量最高。非生物逆境(高温和盐胁迫)和外源激素(脱落酸和水杨酸)处理可以显著改变Sl MAPK9-2的表达水平。启动子预测分析也发现,Sl MAPK9-2启动子区含有大量响应病原菌、激素、高温及脱水的顺式作用元件。综上,Sl MAPK9-2可能在番茄逆境胁迫应答中发挥重要调控作用。本研究为进一步探索Sl MAPK9-2的生物学功能及作用机制奠定了基础。

半边旗提取物6F抑制HL-6 0细胞蛋白激酶C活性(英文)

目的 探讨半边旗提取物 6F的细胞毒作用及诱导DNA片段化与蛋白激酶C(PKC)信号转导途径的关系 ,检测 6F对PKC活性的影响。方法 受试对象为HL 6 0细胞 ,超速离心法获得的胞液 (可溶部分 )及颗粒 (不可溶部分 ,包括细胞膜系统及胞核 )部分用作PKC活性测定。经 0 .4g·L- 1磷脂酰丝氨酸 ,0 .0 4g·L- 1甘油二油酸酯激动剂作用酶粗提物后 ,用液体闪烁计数仪计数 [γ 32 P]ATP参入外源底物的量以测定PKC活性。MTT法测定HL 6 0细胞的活力 ,二苯胺法测定 6F诱导DNA片段化程度。结果 在所测试的浓度范围内 (0 .5～ 312 μmol·L- 1) ,化合物 6F显著抑制胞液及颗粒部分PKC活性 ,最大抑制率达 88.6 % ,呈浓度依赖关系 (胞液部分r =0 .781,P <0 .0 5 ,颗粒部分r =0 .931,P <0 .0 1)。 6F诱导HL 6 0细胞DNA片段化及对细胞的毒性作用可被具有致癌作用的PKC激活剂肉豆蔻酸酯 (PMA ,浓度为 6 5nmol·L- 1)拮抗 ,抑制率分别是 30 %和 4 4% (P <0 .0 1)。PMA单独用使HL 6 0细胞线粒体将MTT还原为甲月赞的能力增强 14 % (P <0 .0 1) ,即增强细胞活力。结论化合物 6F是PKC的抑制剂。 6F对HL 6

谷子SiRLK35基因克隆及功能分析

为探讨谷子(Setaria italica L.)耐旱抗逆机制,解析类受体蛋白激酶(receptor like protein kinase,RLKs)基因功能,进而为培育谷子抗逆新品种提供依据,本文以干旱处理的谷子"豫谷1号"为材料,通过i TRAQ技术筛选到1个干旱响应的类受体蛋白激酶基因,命名为SiRLK35。以谷子RNA反转录的单链cDNA为模板,经PCR扩增获取SiRLK35基因全长序列。应用qRT-PCR方法,对SiRLK35在NaCl、PEG、ABA、GA、Me JA等不同处理下的表达模式进行分析。进一步构建基因原核表达载体pET28a-SiRLK35,结合斑点法对SiRLK35的抗盐能力进行初步评价。同时构建过表达载体p CAMBIA1301P-SiRLK35转化水稻,并对转基因植株抗盐能力进行检测。结果显示:胁迫及激素处理均可不同程度诱导SiRLK35基因的表达;斑点法研究结果显示,在相同NaCl浓度的LB平板上,含有SiRLK35基因的原核表达载体的大肠杆菌菌株生长状态较阴性对照好,SiRLK35具有一定的抗盐能力;获得的转SiRLK35基因水稻植株对盐胁迫的耐受性高于对照。SiRLK35基因对不同胁迫均可以产生响应,但对盐胁迫的响应较为明显,推测该基因可能在谷子的抗盐及抗逆过程中发挥作用。