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来自伤口木质化芦笋的三种差异表达的碱性过氧化物酶。

Three differentially expressed basic peroxidases from wound-lignifying Asparagus officinalis.

作者信息

Holm Kirsten B, Andreasen Per H, Eckloff Reinhard M G, Kristensen Brian K, Rasmussen Søren K

机构信息

Plant Research Department, PRD-301, Risø National Laboratory, PO Box 49, DK-4000 Roskilde, Denmark.

出版信息

J Exp Bot. 2003 Oct;54(391):2275-84. doi: 10.1093/jxb/erg253. Epub 2003 Aug 28.

Abstract

The activity of ionically bound peroxidases from an asparagus spear increased from 5-24 h post-harvest. Isoelectric focusing showed that the post-harvest increase of the total peroxidase activity was due to the increase of several distinct isoperoxidases. Concomitantly, a decrease in the activity of two anionic peroxidases was observed. Peroxidases with pI 5.9, 6.4 and 9.2 were detected only at 24 h post-harvest, whereas four peroxidases, with pI 8.7, 8.1, 7.4, and 6.7, detected throughout the time-course, increased in their activity. Histochemical staining demonstrated that lignin and peroxidase activity were located in the vascular bundles throughout the period of measurement. Lignin was detected in the cell walls of the protoxylem in the vascular bundles of the asparagus stem. A cDNA library of mRNA isolated from asparagus spears 24 h post-harvest was screened for peroxidases using homologous and heterologous probes. Three clones were isolated and the corresponding mature asparagus peroxidases displayed 70%, 76% and 81% amino acid sequence identity to each other. These new asparagus peroxidases are typical class III plant peroxidases in terms of conserved regions with a calculated pI >9.2, which is consistent with most basic peroxidases. One of the genes was shown to be a constitutively expressed single-copy gene, whereas the others showed an increased expression at post-harvest. The highest similarity in the amino acid sequence (71-77%) was found in peroxidases from roots of winter grown turnip TP7, to Arabidopsis AtP49, to an EST sequence from cotton fibres and to TMV-infected tobacco.

摘要

芦笋茎尖离子结合过氧化物酶的活性在采后5 - 24小时内升高。等电聚焦显示,采后总过氧化物酶活性的增加是由于几种不同的同功过氧化物酶增加所致。同时,观察到两种阴离子过氧化物酶的活性降低。pI为5.9、6.4和9.2的过氧化物酶仅在采后24小时检测到,而在整个时间进程中检测到的四种pI为8.7、8.1、7.4和6.7的过氧化物酶活性增加。组织化学染色表明,在整个测量期间,木质素和过氧化物酶活性都位于维管束中。在芦笋茎维管束的原生木质部细胞壁中检测到木质素。使用同源和异源探针,对采后24小时从芦笋茎尖分离的mRNA的cDNA文库进行过氧化物酶筛选。分离出三个克隆,相应的成熟芦笋过氧化物酶彼此之间的氨基酸序列同一性为70%、76%和81%。就保守区域而言,这些新的芦笋过氧化物酶是典型的III类植物过氧化物酶,计算出的pI >9.2,这与大多数碱性过氧化物酶一致。其中一个基因被证明是组成型表达的单拷贝基因,而其他基因在采后表达增加。在来自冬季种植的芜菁根TP7的过氧化物酶、拟南芥AtP49、棉纤维的一个EST序列以及感染TMV的烟草中,发现氨基酸序列的最高相似性为71 - 77%。

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