杀虫遗传工程荧光假单胞菌IPP202部分生物学特性

对遗传工程荧光假单胞菌IPP202进行了质粒稳定性检 测、抑菌活性测定、在棉花根部和叶面定殖能力分析、杀虫蛋白抗紫外能力检测及田间杀虫 活性测定等试验。结果表明,工程菌与出发菌株P303相比,其抑菌、定殖等有益于植物的优 良特性未发生显著变化;经过连续培养和连续稀释培养后工程菌的质粒都非常稳定;广波长 紫外线照射2 h后,苏云金芽胞杆菌(Bacillus thuringiensis,简称Bt)由于裸露的伴 孢晶体杀虫蛋白受紫外线破坏因而杀虫活性大大下降,而荧光假单胞菌工程菌的活性变化不 大;IPP202田间杀虫活性与Bt野生菌株接近。工程菌有望解决Bt本身存在的杀虫蛋白多以裸 露晶体的形式存在而易受紫外线破坏的弱点,同时也发挥了P303菌株在多种植物上定殖能力 的优点,使其具有在植物周围大量繁殖而直到杀虫作用的优势。通过进一步研究,将有望构 建成更有实用价值的工程菌。     

小熊猫染色体异染色质的显示

以培养的小熊猫外周淋巴细胞为实验材料,结合Ｃ－显带技术及ＣＭＡ３／ＤＡ／ＤＡＰＩ三竽荧光杂色的方法,对小熊猫的染色体组型、Ｃ－带带型及ＣＭＡ３／ＤＡ／ＤＡＰＩ荧光带带型进行了研究,发现：（１）经Ｃ－显带技术处理,可在小熊猫染色体上呈现出一种极为独特的Ｃ－带带型。在多数染色体上可见到丰富的插入Ｃ－带及端粒Ｃ－带。而着丝区仅显示弱阳性Ｃ－带;（２）除着丝粒区外,ＣＭＡ３诱导的大多数强荧光带纹与Ｃ－阳性     

Dexamethasone-inducible green fluorescent protein gene expression in transgenic plant cells

Genomic research has made a large number of sequences of novel genes or expressed sequence tags available. To investigate functions of these genes, a system for conditional control of gene expression would be a useful tool. Inducible transgene expression that uses green fluorescent protein gene (gfp) as a reporter gene has been investigated in transgenic cell lines of cotton (COT; Gossypium hirsutum L.), Fraser fir [FRA; Abies fraseri (Pursh) Poir], Nordmann fir (NOR; Abies nordmanniana Lk.), and rice (RIC; Oryza sativa L. cv. Radon). Transgenic cell lines were used to test the function of the chemical inducer dexamethasone. Inducible transgene expression was observed with fluorescence and confocal microscopy, and was confirmed by northern blot analyses. Dexamethasone at 5 mg/L induced gfp expression to the nearly highest level 48 h after treatment in COT, FRA, NOR, and RIC. Dexamethasone at 10 mg/L inhibited the growth of transgenic cells in FRA and NOR, but not COT and RIC. These results demonstrated that concentrations of inducer for optimum inducible gene expression system varied among transgenic cell lines. The inducible gene expression system described here was very effective and could be valuable in evaluating the function of novel gene.     

Soluble expression and characterization of a GFP-fused pea actin isoform（PEAc1）

A pea actin isoform PEAcl with green fluorescent protein (GFP) fusion to its C-terminus and His-tag to its Nterminus, was expressed in prokaryotic cells in soluble form, and highly purified with Ni-Chelating Sepharose^TM Fast Flow column. The purified fusion protein (PEAcl-GFP) efficiently inhibited DNase I activities before polymerization,and activated the myosin Mg-ATPase activities after polymerization. The PEAcl-GFP also polymerized into green fluorescent filamentous structures with a critical concentration of 0.75μM. These filamentous structures were labeled by TRITC-phalloidin, a specific agent for staining actin microfilaments, and identified as having 9 nm diameters by negative staining. These results indicated that PEAc 1 preserved the essential characteristics of actin even with His-tag and GFP fusion, suggesting a promising potential to use GFP fusion protein in obtainning soluble plant actin isoform to analyze its physical and biochemical properties in vitro. The PEAcl-GFP was also expressed in tobacco BY2 cells,which offers a new pathway for further studying its distribution and function in vivo.     

加工产品中转基因玉米Bt11成分实时荧光PCR定量(性)检测

实验在玉米自身基因和外源基因的边界序列之间设计了具有品种和品系特异性的引物和探针 ,并以实时荧光PCR技术 ,建立了加工产品中转基因玉米Bt1 1成分品系鉴定检测和定量检测的方法。实验对加热条件和时间对检测转基因成分的影响作了探讨 ,并检测了部分市售食品和饲料。检测结果发现 ,加热时间温度越高、时间越长 ,对转基因成分定量检测的影响越大 ;在所检测的样品中可以检测出转基因玉米Bt1 1成分 ,有些样品还同时检出其他转基因成分。本研究实验建立的方法 ,可以用于加工产品中转基因成分的定量检测 ,也可以用于定性检测 ,或作为常规PCR定性检测后的确证实验方法。     

砂仁叶片光破坏的防御

报告了生长于热带林窗向阳处砂仁叶片叶绿素荧光参数的日变化,及阻止卷叶和用二硫苏糖醇(DTT)处理对它的影响.受强光照射,砂仁叶片迅速卷起.在雾天上午光强还相当弱(低于100μmol m-2s-1)时,砂仁叶片就发生光抑制,中午最重,下午当光强减弱时,光抑制逐渐得到缓解.其热耗散(qN、NPQ)随光强的升高而增加,且下午仍在缓慢增加.阻止卷叶使强光下砂仁叶片光抑制加剧,F0、NPQ升高.DTT处理也使光抑制加剧,F0升高,且使PSⅡ反应中心发生可逆失活.夜间2300各处理的荧光参数基本恢复.卷叶、叶黄素循环和PSⅡ可逆失活3种保护机制在同种植物中依次启动的现象尚属少见.     

苏云金芽孢杆菌cry1基因在荧光假单胞菌Pfx-18中的表达特性

用DIG标记的cry1Aa基因EcoRI-F片段的RNA探针,对筛选的鳞翅目高毒力菌株的质粒进行Southern分析,将cry基因定位在39．3MD质粒上。该质粒经HindⅢ酶解,用同样探针进行杂交,呈现6．5kb和7．1kb两条阳性带,其中7．1kb片段的杂交强度明显高于6．5kb片段。将7．1kb片段与多寄主质粒pSUP106连接,转化荧光假单胞菌Pfx－18,获得克隆子LZP-1。克隆基因用PCR鉴定,显示典型的cry1Ab谱带。经SDS-PAGE分析,克隆株表达66kD杀虫晶体蛋白和一些小分子多肽。其发酵液稀释1000倍对三龄小菜蛾幼虫的致死率为33％。     

应用FISH技术鉴定一个小冰麦易位系

以生物素（ｂｉｏｔｉｎ１６ｄＵＴＰ）标记的天蓝冰草（Ａｇｒｏｐｙｒｏｎｉｎｔｅｒｍｅｄｉｕｍ（Ｈｏｓｔ）Ｐ．Ｂ．＝Ｅｌｙｔｒｉｇｉａｉｎｔｅｒｍｅｄｉａ（Ｈｏｓｔ）Ｎｅｖｓｋｉ＝Ｔｈｉｎｏｐｙｒｕｍｉｎｔｅｒｍｅｄｉｕｍ（Ｈｏｓｔ）ＢａｒｋｗｏｒｔｈａｎｄＤｅｗｅｙ）染色体组ＤＮＡ为探针,普通小麦（ＴｒｉｔｉｃｕｍａｅｓｔｉｖｕｍＬ．）“中国春”ＤＮＡ为封闭,用荧光原位杂交（ＦＩＳＨ）技术对小冰麦３３号进行检测。结果表明：在一对染色体的端部显现出绿色荧光,这说明小冰麦３３号携带外源基因的冰草染色体片段位于小麦染色体端部,而且易位的染色体片段是较小的。从ＤＮＡ水平直接证明小冰麦３３是一个冰草染色体片段易位到小麦染色体端部的易位系。     

绿色荧光蛋白基因在水稻细胞中的高效表达

绿色荧光蛋白基因在水稻细胞中的高效表达＠许新萍＠黄粤＠卫剑文＠李宝健￥中山大学生物工程研究中心绿色荧光蛋白,水稻,瞬间表达,β－葡糖苷酸酶绿色荧光蛋白基因在水稻细胞中的高效表达许新萍黄粤卫剑文李宝健（中山大学生物工程研究中心广州５１０２７５）关键词绿色荧...