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Nectarin IV a Potent Endoglucanase Inhibitor Secreted into the Nectar of Ornamental Tobacco Plants. Isolation Cloning and Characterization

机译:Nectarin IV一种分泌到观赏烟草植物花蜜中的有效内切葡聚糖酶抑制剂。分离克隆和表征

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摘要

We have isolated and characterized the Nectarin IV (NEC4) protein that accumulates in the nectar of ornamental tobacco plants (Nicotiana langsdorffii × Nicotiana sanderae var LxS8). This 60-kD protein has a blocked N terminus. Three tryptic peptides of the protein were isolated and sequenced using tandem mass spectroscopy. These unique peptides were found to be similar to the xyloglucan-specific fungal endoglucanase inhibitor protein (XEGIP) precursor in tomato (Lycopersicon esculentum) and its homolog in potato (Solanum tuberosum). A pair of oligonucleotide primers was designed based on the potato and tomato sequences that were used to clone a 1,018-bp internal piece of nec4 cDNA from a stage 6 nectary cDNA library. The remaining portions of the cDNA were subsequently captured by 5′ and 3′ rapid amplification of cDNA ends. Complete sequencing of the nec4 cDNA demonstrated that it belonged to a large family of homologous proteins from a wide variety of angiosperms. Related proteins include foliage proteins and seed storage proteins. Based upon conserved identity with the wheat (Triticum aestivum) xylanase inhibitor TAXI-1, we were able to develop a protein model that showed that NEC4 contains additional amino acid loops that are not found in TAXI-1 and that glycosylation sites are surface exposed. Both these loops and sites of glycosylation are on the opposite face of the NEC4 molecule from the site that interacts with fungal hemicellulases, as indicated by homology to TAXI-I. NEC4 also contains a region homologous to the TAXI-1 knottin domain; however, a deletion in this domain restructures the disulfide bridges of this domain, resulting in a pseudoknottin domain. Inhibition assays were performed to determine whether purified NEC4 was able to inhibit fungal endoglucanases and xylanases. These studies showed that NEC4 was a very effective inhibitor of a family GH12 xyloglucan-specific endoglucanase with a Ki of 0.35 nm. However, no inhibitory activity was observed against other family GH10 or GH11 xylanases. The patterns of expression of the NEC4 protein indicate that, while expressed in nectar at anthesis, it is most strongly expressed in the nectary gland after fertilization, indicating that inhibition of fungal cell wall-degrading enzymes may be more important after fertilization than before.
机译:我们已经分离并鉴定了在观赏烟草植物(Nicotiana langsdorffii×Nicotiana sanderae var LxS8)的花蜜中积累的油桃IV(NEC4)蛋白。该60 kD蛋白的N末端受阻。分离出蛋白质的三个胰蛋白酶肽,并使用串联质谱法进行测序。发现这些独特的肽类似于番茄(Lycopersicon esculentum)中的木葡聚糖特异性真菌内切葡聚糖酶抑制剂蛋白(XEGIP)前体,以及马铃薯中的同源物(Solanum tuberosum)。根据马铃薯和番茄序列设计了一对寡核苷酸引物,该序列用于从第6阶段蜜腺cDNA文库克隆一个1,018-bp内部nec4 cDNA。随后通过5'和3'快速扩增cDNA末端捕获cDNA的其余部分。 nec4 cDNA的完整测序表明,它属于来自各种被子植物的一大类同源蛋白。相关蛋白包括叶子蛋白和种子贮藏蛋白。基于与小麦(Triticum aestivum)木聚糖酶抑制剂TAXI-1的保守身份,我们能够开发一种蛋白质模型,该模型显示NEC4包含TAXI-1中未发现的其他氨基酸环,并且糖基化位点是表面暴露的。这些环和糖基化位点均位于NEC4分子与与真菌半纤维素酶相互作用的位点相反的面上,如与TAXI-1的同源性所示。 NEC4还包含一个与TAXI-1结蛋白域同源的区域。然而,该结构域中的缺失重组了该结构域的二硫键,导致了假结蛋白结构域。进行抑制测定以确定纯化的NEC4是否能够抑制真菌内切葡聚糖酶和木聚糖酶。这些研究表明,NEC4是GH12木葡聚糖特异性内切葡聚糖酶家族的非常有效的抑制剂,Ki为0.35 nm。然而,未观察到针对其他家族GH10或GH11木聚糖酶的抑制活性。 NEC4蛋白的表达模式表明,虽然花蜜在花蜜中表达,但受精后在腺体中表达最强,这表明受精后抑制真菌细胞壁降解酶可能比以前更重要。

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