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首页> 外文期刊>Transgenic research >Visualisation of plastids in endosperm, pollen and roots of transgenic wheat expressing modified GFP fused to transit peptides from wheat SSU RubisCO, rice FtsZ and maize ferredoxin III proteins.
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Visualisation of plastids in endosperm, pollen and roots of transgenic wheat expressing modified GFP fused to transit peptides from wheat SSU RubisCO, rice FtsZ and maize ferredoxin III proteins.

机译:可视化的胚乳,花粉和表达修饰的GFP的转基因小麦根中的质体与小麦SSU RubisCO,水稻FtsZ和玉米铁氧还蛋白III蛋白的转运肽融合。

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摘要

The ability to target marker proteins to specific subcellular compartments is a powerful research tool to study the structure and development of organelles. Here transit sequences from nuclear-encoded, plastid proteins, namely rice FtsZ, maize non-photosynthetic ferredoxin III (FdIII) and the small subunit of RubisCO were used to target a modified synthetic GFP (S65G, S72A) to plastids. The localisations of the fusion proteins expressed in transgenic wheat plants and under the control of the rice actin promoter were compared to an untargeted GFP control. GFP fluorescence was localised to non-green plastids in pollen, roots and seed endosperm and detected in isolated leaf chloroplasts using a GFP-specific antibody. Transit peptides appeared to influence the relative fluorescence intensities of plastids in different tissues. This is consistent with differential targeting and/or turnover of GFP fusion proteins in different plastid types. Replacement of GFP sequences with alternative coding regions enables immediate applications of our vectors for academic research and commercial applications.
机译:将标记蛋白靶向特定亚细胞区室的能力是研究细胞器结构和发育的强大研究工具。在这里,来自核编码的质体蛋白的转运序列,即水稻FtsZ,玉米非光合铁氧还蛋白III(FdIII)和RubisCO的小亚基被用于将修饰的合成GFP(S65G,S72A)靶向质体。将在转基因小麦植株中表达并在水稻肌动蛋白启动子控制下的融合蛋白的定位与未靶向的GFP对照进行了比较。 GFP荧光定位于花粉,根和种子胚乳中的非绿色质体,并使用GFP特异性抗体在分离的叶绿体中检测到。转运肽似乎会影响不同组织中质体的相对荧光强度。这与不同质体类型中GFP融合蛋白的差异靶向和/或更新一致。用其他编码区替换GFP序列可将我们的载体立即用于学术研究和商业应用。

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