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Phytosulfokine(PSK)is a new peptide plant hormone,which was isolated in the conditioned medium of cultures derived from both monoco-tyledonous and dicotyledonous plants,such as Asparagus officinalis mesophyll[1],rice[2],zinnia[3],and carrot[4].PSK has two types of structure:PSK-αand PSK-β.The former is a sulfated pentapeptide[H-Tyr(SO3H)-Ile-Tyr(SO3H)-Thr-Gln-OH],the latter is a sulfated terapeptide[H-Tyr(SO3H)-Ile-Tyr(SO3H)-Thr-OH].Both are heat-stable,susceptible to pronase… 相似文献
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为提高紫花苜蓿(Medicago sativa)的抗逆性,利用在朝鲜碱茅(Puccinellia chinampoensis)已克隆的Pu P5CS基因成功构建了p CAMBIA3300-Pu P5CS表达载体,以子叶为外植体,通过农杆菌介导共培养法转化紫花苜蓿"公农5号"(M.sativa cv.Gongnong No.5),并以2.0 mg·L-1的草铵膦进行筛选,抗性愈伤组织诱导率为22.4%,经草铵膦筛选的植株进行PCR检测和RT-PCR检测。结果显示,共获得11株转化植株,表明Pu P5CS基因已转入T0紫花苜蓿植株,且能够在RNA水平上正常表达。 相似文献
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以香蕉(Musa spp.)品种‘天宝蕉’(Musa spp.,AAA类群)为试材,对以根癌农杆菌介导法的香蕉遗传转化体系进行较全面的研究,并以该系统进行了ACS反义基因转化香蕉的研究。结果表明:不经预培养的香蕉茎尖横切薄片,侵染前用附加0.1 mg/L甘露醇的高渗固体培养基前处理4 h,农杆菌重悬液浓度为OD600在1.0左右,重悬液中含100 g/L蔗糖,接菌时间为10~15 min,于26℃黑暗条件下共培养4 d,共培养培养基pH值为5.8是较为适合的转化条件;采用附加100 mg/L卡那霉素、2 mg/L AgNO3筛选培养基对共培养后的香蕉横切薄片进行筛选,共获得5个转ACS反义基因的抗性芽系;经GUS组织化学法及PCR检测,gus基因已整合进香蕉基因组。 相似文献
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HUANG Jia-quan SUN Zhong-hai 《中国农业科学(英文版)》2005,4(9):714-720
The Arabidopsis ICEI (inducer of CBF expression 1) gene was cloned through RT-PCR of Arabidopsis cDNAs and introduced into the lemon (Citrus Limon (L.) Burm. F. cv. Eureka) genome using Agrobacterium-mediated transformation method. Epicotyl segments from in vitro grown lemon seedlings were co-cultivated with A. tumefaciens strain EHA 105 carrying the binary plasmid pMVICE1, whose T-DNA region contain ICEI gene driven by 35S CaMV promoter. Among 320 epicotyl segments inoculated, 71 explants responded and regenerated 51 elongated shoots. These shoots were subjected to an extra month of kanamycin exposure. In this way, the number of escapes reduced. Thirteen of 31 survived shoots formed roots and 7 were tested positive using PCR technique. Southern blot analyses confirmed PCR results and demonstrated that more than two copies of the ICE1 gene were integrated into the lemon genome. 相似文献
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【目的】将具有广谱抗病性的hrpZpsta基因导入大豆,为培育抗灰斑病的转基因大豆新品系奠定基础。【方法】采用农杆菌介导法,以大豆子叶节为受体,将具有广谱抗性的hrpZpsta基因转入大豆品种"吉林30"中,以耐盐基因badh作为筛选标记性基因,经过抗性筛选,对转基因植株进行PCR检测、Southern杂交和RT-PCR检测分析。【结果】确定的NaCl筛选浓度为200mmol/L。对T1、T2和T3代转基因植株进行PCR检测,得到T1代阳性植株30株,T2代45株,T3代284株,说明外源hrpZpsta基因在转基因后代中能够遗传。Southern杂交结果表明,外源目的基因hrpZpsta已经整合进大豆基因组中,且整合位点不尽相同。RT-PCR结果表明,hrpZpsta基因在受体大豆中获得表达。【结论】获得了hrpZpsta基因遗传表达的T3代转基因大豆株系。 相似文献
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以辣椒品种'B162'为试材,探讨了通过根癌农杆菌介导法将黄瓜花叶病毒外壳蛋白(CMV-CP)基因转化辣椒的适宜条件.结果表明,将辣椒带柄子叶进行预培养2 d后,用D600 nm为0.3的根癌农杆菌菌液浸泡7 min,再经过共培养2 d后转移到筛选分化培养基中进行培养,有利于获得辣椒抗性不定芽.通过对获得的10株抗性不定芽进行PCR检测,其中有2株扩增出目的条带,初步证明CMV-CP基因已经转入辣椒不定芽中. 相似文献