[Objective]The aim was to explore the molecular mechanism of plant resistance to various stress response.[Method]The expression of LeWRKY1 in tomato seedlings under treatment with B.cinerea,exogenous JA and SA were ex...[Objective]The aim was to explore the molecular mechanism of plant resistance to various stress response.[Method]The expression of LeWRKY1 in tomato seedlings under treatment with B.cinerea,exogenous JA and SA were explored by real time quantitative RT-PCR technology.[Result]JA induced the expression of LeWRKY1,but SA did not.LeWRKY1 expression was up-regulated under B.cinerea infection.[Conclusion]LeWRKY1 might be involved in the tomato defense response to B.cinerea through JA dependent but SA independent signal pathway.展开更多
[Objective] This study was carried out to determine the induction effect of jasmonic acid(JA)on powdery mildew resistance in wheat,the activation effect on the expressions of plant disease resistance related genes,a...[Objective] This study was carried out to determine the induction effect of jasmonic acid(JA)on powdery mildew resistance in wheat,the activation effect on the expressions of plant disease resistance related genes,and to investigate the relationship between the induced resistance and the gene expression patterns.[Method] Three powdery mildew susceptible cultivars of "Chinese Spring","Pumai 9" and "Zhoumai 18" typically representing different phenotypes in the field were employed.The powdery mildew was assessed by detached leaf assay,and real time quantitative RT-PCR was used to determine the expression patterns of 9 disease resistance related genes of PR1(PR1.1),PR2(β,1-3 glucanase),PR3(chitinase),PR4(wheatwin1),PR5(thaumatin-like protein),PR9(TaPERO,peroxidase),PR10,TaGLP2a(germin-like)and Ta-JA2(jasmonate-induced protein)in leaf of the three cultivars.[Result] MeJA application enhanced the powdery mildew resistances of "Chinese Spring","Pumai 9" and "Zhoumai 18".The induced powdery mildew resistance could be detected from 12 h to 96 h after MeJA treatment,and the peak value was at 24 h.Though there were differences between the three cultivars,MeJA significantly effect on the expressions of the 8 disease resistance related genes except TaGLP2a,and the peak values were at 12 h,24 h or 48 h after treatments.The strongest activation of MeJA was on PR9 and PR1 that their expressions could reach more than 100 times of the untreated samples.MeJA strongly activated PR2、PR4、PR5、PR3、PR10 and Ta-JA2,their expression could reach 10 to 70 times,and there was almost no activation effect on TaGLP2a.The induced powdery mildew resistance positively correlated with the induced expressions of the 8 disease related genes.[Conclusion] The induced powdery mildew resistance positively correlated with the induced expressions of the disease related genes.Jasmonate signalling plays a role in defence against Blumeria graminis f.sp.tritici.and future manipulation of this pathway may improve powdery mildew resistance in wheat.展开更多
[Objective]The study was to analyze the expression of the deletion fragments from the promoter of a glycosyltransferase gene induced both by MeJA and SA cloned from tobacco W38(sm-Ngt) in transgenic tobacco plants.[...[Objective]The study was to analyze the expression of the deletion fragments from the promoter of a glycosyltransferase gene induced both by MeJA and SA cloned from tobacco W38(sm-Ngt) in transgenic tobacco plants.[Method]Using T1 seedlings of sm-Ngt transgenic tobacco lines containing Gus gene controlled by five 5' flank deletion promoter fragments different in length as experimental materials,GUS histochemical staining and fluorometric analysis of T1 seedlings treated with MeJA and SA for 16 h were conducted to analyze the effect of MeJA and SA treatment on the expression of 5' flank deletion promoter fragments.[Result]Of five 5' flank deletion promoter fragments transgenic plant lines,30 d old T1 seedlings containing 220-0 bp promoter fragment performed worst in GUS staining(showing least staining spots),those containing-524-0 bp and-468-0 bp promoter fragment both performed best.In the plants not treated with MeJA and SA,activities of GUS driven by-524-0 bp and-468-0 bp deletion promoter fragments were enormously higher than that driven by-1 150-0,-800-0 or-220 0 bp,and which were proved to be not resulted from insert copy number by Southern blot.For GUS expression,promoter fragment-800-0 bp expression was doubly induced by both MeJA and SA,while fragment-1 150-0 was induced by MeJA.[Conclusion]There are activity enhancement elements within-524--220 bp of the sm-Ngt in promoter and activity down regulation elements within-1 150--524 bp region,as well as MeJA and SA doubly inducing activity regulation elements in this promoter.展开更多
The cDNA sequence of Capal gene was cloned from Capsicum chinense Jacq by RT-PCR and sequenced. Bioinformatics analysis showed that Capal en- codes a putative polypeptide of 683 amino acids with a calculated molecular...The cDNA sequence of Capal gene was cloned from Capsicum chinense Jacq by RT-PCR and sequenced. Bioinformatics analysis showed that Capal en- codes a putative polypeptide of 683 amino acids with a calculated molecular mass of 74.2 kD and a theoretical pl of 6.9. Multiple sequence alignments and phyloge- netic tree analyses showed that Capal protein of C. chinense is similar to that of Capsicum annuum var. conoides, with an overall sequence similarity of 96%. The prokaryotic expression vector pET-32a-pal was constructed and induced to express in E. coil BL21. The SDS-PAGE analysis showed that the relative molecular mass of the induced new protein is about 74 kD, which was basically identical with that predicted by DNAMAN software (74.3 kD), Real-time PCR analysis showed that ex- ogenous jasmonic acid (JA) promoted pal expression. The accumulation of capsaicin in pepper was analyzed by high performance liquid chromatography (HPLC), and the results indicated that exogenous jasmonic acid (JA) can promote the synthesis of capsaicin. This study will provide valuable experimental basis for the research of transcription regulation and explaining the gene function of pal.展开更多
To explore the regulatory effects of jasmonic acid (JA) on the expression of the genes involved in capsaicin biosynthesis pathway, the mRNA expression of the genes was determined by fluorescence-based quantitative P...To explore the regulatory effects of jasmonic acid (JA) on the expression of the genes involved in capsaicin biosynthesis pathway, the mRNA expression of the genes was determined by fluorescence-based quantitative PCR 0, 4, 12, 24 and 48 h after chili peppers (Capsicum annuum var. conoides) were treated with 100 μmol/L JA, and the content of capsaicin was measured by high performance liquid chromatography (HPLC) 0, 1, 3, 6, 10 and 15 d after JA treatment. The results showed that JA upregulated the mRNA levels of pal, C4h, Comt, 4Cl, Hct, Paint, Bcat, FatA and pun1 in chili pepper, thus promoting the synthesis of capsaicin to different extents.展开更多
基金Supported by Beijing Nature Science Foundation(5102015)~~
文摘[Objective]The aim was to explore the molecular mechanism of plant resistance to various stress response.[Method]The expression of LeWRKY1 in tomato seedlings under treatment with B.cinerea,exogenous JA and SA were explored by real time quantitative RT-PCR technology.[Result]JA induced the expression of LeWRKY1,but SA did not.LeWRKY1 expression was up-regulated under B.cinerea infection.[Conclusion]LeWRKY1 might be involved in the tomato defense response to B.cinerea through JA dependent but SA independent signal pathway.
基金Supported by The Key Project of Science and Technology of HenanProvince(102102110040)Innovation Scientists and the Innovation Fund for Outstanding Scholars of Henan Province(104200510013)~~
文摘[Objective] This study was carried out to determine the induction effect of jasmonic acid(JA)on powdery mildew resistance in wheat,the activation effect on the expressions of plant disease resistance related genes,and to investigate the relationship between the induced resistance and the gene expression patterns.[Method] Three powdery mildew susceptible cultivars of "Chinese Spring","Pumai 9" and "Zhoumai 18" typically representing different phenotypes in the field were employed.The powdery mildew was assessed by detached leaf assay,and real time quantitative RT-PCR was used to determine the expression patterns of 9 disease resistance related genes of PR1(PR1.1),PR2(β,1-3 glucanase),PR3(chitinase),PR4(wheatwin1),PR5(thaumatin-like protein),PR9(TaPERO,peroxidase),PR10,TaGLP2a(germin-like)and Ta-JA2(jasmonate-induced protein)in leaf of the three cultivars.[Result] MeJA application enhanced the powdery mildew resistances of "Chinese Spring","Pumai 9" and "Zhoumai 18".The induced powdery mildew resistance could be detected from 12 h to 96 h after MeJA treatment,and the peak value was at 24 h.Though there were differences between the three cultivars,MeJA significantly effect on the expressions of the 8 disease resistance related genes except TaGLP2a,and the peak values were at 12 h,24 h or 48 h after treatments.The strongest activation of MeJA was on PR9 and PR1 that their expressions could reach more than 100 times of the untreated samples.MeJA strongly activated PR2、PR4、PR5、PR3、PR10 and Ta-JA2,their expression could reach 10 to 70 times,and there was almost no activation effect on TaGLP2a.The induced powdery mildew resistance positively correlated with the induced expressions of the 8 disease related genes.[Conclusion] The induced powdery mildew resistance positively correlated with the induced expressions of the disease related genes.Jasmonate signalling plays a role in defence against Blumeria graminis f.sp.tritici.and future manipulation of this pathway may improve powdery mildew resistance in wheat.
基金Supported by Natural Science Foundation of Hubei Province(2004ABA123)~~
文摘[Objective]The study was to analyze the expression of the deletion fragments from the promoter of a glycosyltransferase gene induced both by MeJA and SA cloned from tobacco W38(sm-Ngt) in transgenic tobacco plants.[Method]Using T1 seedlings of sm-Ngt transgenic tobacco lines containing Gus gene controlled by five 5' flank deletion promoter fragments different in length as experimental materials,GUS histochemical staining and fluorometric analysis of T1 seedlings treated with MeJA and SA for 16 h were conducted to analyze the effect of MeJA and SA treatment on the expression of 5' flank deletion promoter fragments.[Result]Of five 5' flank deletion promoter fragments transgenic plant lines,30 d old T1 seedlings containing 220-0 bp promoter fragment performed worst in GUS staining(showing least staining spots),those containing-524-0 bp and-468-0 bp promoter fragment both performed best.In the plants not treated with MeJA and SA,activities of GUS driven by-524-0 bp and-468-0 bp deletion promoter fragments were enormously higher than that driven by-1 150-0,-800-0 or-220 0 bp,and which were proved to be not resulted from insert copy number by Southern blot.For GUS expression,promoter fragment-800-0 bp expression was doubly induced by both MeJA and SA,while fragment-1 150-0 was induced by MeJA.[Conclusion]There are activity enhancement elements within-524--220 bp of the sm-Ngt in promoter and activity down regulation elements within-1 150--524 bp region,as well as MeJA and SA doubly inducing activity regulation elements in this promoter.
基金Supported by Innovation Fund of Undergraduate Education in Jilin University(2012A82221)Jilin Provincial Natural Science and Technology Foundation(20101568)~~
文摘The cDNA sequence of Capal gene was cloned from Capsicum chinense Jacq by RT-PCR and sequenced. Bioinformatics analysis showed that Capal en- codes a putative polypeptide of 683 amino acids with a calculated molecular mass of 74.2 kD and a theoretical pl of 6.9. Multiple sequence alignments and phyloge- netic tree analyses showed that Capal protein of C. chinense is similar to that of Capsicum annuum var. conoides, with an overall sequence similarity of 96%. The prokaryotic expression vector pET-32a-pal was constructed and induced to express in E. coil BL21. The SDS-PAGE analysis showed that the relative molecular mass of the induced new protein is about 74 kD, which was basically identical with that predicted by DNAMAN software (74.3 kD), Real-time PCR analysis showed that ex- ogenous jasmonic acid (JA) promoted pal expression. The accumulation of capsaicin in pepper was analyzed by high performance liquid chromatography (HPLC), and the results indicated that exogenous jasmonic acid (JA) can promote the synthesis of capsaicin. This study will provide valuable experimental basis for the research of transcription regulation and explaining the gene function of pal.
基金Supported by the Innovation Fund for Undergraduate of Jilin University(2016A82361)~~
文摘To explore the regulatory effects of jasmonic acid (JA) on the expression of the genes involved in capsaicin biosynthesis pathway, the mRNA expression of the genes was determined by fluorescence-based quantitative PCR 0, 4, 12, 24 and 48 h after chili peppers (Capsicum annuum var. conoides) were treated with 100 μmol/L JA, and the content of capsaicin was measured by high performance liquid chromatography (HPLC) 0, 1, 3, 6, 10 and 15 d after JA treatment. The results showed that JA upregulated the mRNA levels of pal, C4h, Comt, 4Cl, Hct, Paint, Bcat, FatA and pun1 in chili pepper, thus promoting the synthesis of capsaicin to different extents.
