NtCP56, a new cysteine protease in Nicotiana tabacum L., involved in pollen grain development

Zhang, Xiaomei; Ying, Wang; Lv, Xiao-Meng; Li, Hui; Sun, Peter P.; Lu, Hai; Li, Fenglan

doi:10.1093/jxb/erp022

Cited by 34 publications

(39 citation statements)

References 41 publications

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“…CP gene identification has occurred in several plant sources, such as Mesembryanthemum crystallinum (Forsthoefel et al, 1998), Daucus carota (Mitsuhashi et al, 2004), and C. candamarcensis (Pereira et al, 2001). Over-expression of CP genes from plant sources, like C. papaya (Taylor et al, 1999), Ipomoea batatas (Chen et al, 2009;2010), Nicotiana tabacum (Beyene et al, 2006;Zhang et al, 2009), and C. candamarcensis (Corrêa et al, 2011), has also been reported and shown to be encouraging examples of the aims presented in this study. The main objective of this research was to identify the gene sequences coding for the proteases that comprise the latex of J. mexicana.…”

Section: Introductionsupporting

confidence: 52%

Isolation of cDNA from Jacaratia mexicana encoding a mexicain-like cysteine protease gene

Ramos-Martinez

Herrera-Ramírez

Badillo-Corona

et al. 2012

Gene

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Section: Introductionsupporting

confidence: 52%

Isolation of cDNA from Jacaratia mexicana encoding a mexicain-like cysteine protease gene

Ramos-Martinez

Herrera-Ramírez

Badillo-Corona

et al. 2012

Gene

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“…The expression, extraction, purification, and renaturation of the CEP1 protein were performed according to the procedure described by Zhang et al (2009).…”

Section: Molecular Cloning and Plasmid Constructionmentioning

confidence: 99%

“…The expression, extraction, purification, and renaturation of the CEP1 peptide were performed according to the procedures described by Zhang et al (2009).The purified recombinant peptide (5 mg) was used to immunize rabbits at 3-week intervals. The specificity of the CEP1 antibody was confirmed by hybridization with a membrane blotted with protein extracts from the buds of Arabidopsis (Supplemental Figure 7).…”

Section: Cep1 Immunolocalizationmentioning

confidence: 99%

The Cysteine Protease CEP1, a Key Executor Involved in Tapetal Programmed Cell Death, Regulates Pollen Development in Arabidopsis

et al. 2014

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Tapetal programmed cell death (PCD) is a prerequisite for pollen grain development in angiosperms, and cysteine proteases are the most ubiquitous hydrolases involved in plant PCD. We identified a papain-like cysteine protease, CEP1, which is involved in tapetal PCD and pollen development in Arabidopsis thaliana. CEP1 is expressed specifically in the tapetum from stages 5 to 11 of anther development. The CEP1 protein first appears as a proenzyme in precursor protease vesicles and is then transported to the vacuole and transformed into the mature enzyme before rupture of the vacuole. cep1 mutants exhibited aborted tapetal PCD and decreased pollen fertility with abnormal pollen exine. A transcriptomic analysis revealed that 872 genes showed significantly altered expression in the cep1 mutants, and most of them are important for tapetal cell wall organization, tapetal secretory structure formation, and pollen development. CEP1 overexpression caused premature tapetal PCD and pollen infertility. ELISA and quantitative RT-PCR analyses confirmed that the CEP1 expression level showed a strong relationship to the degree of tapetal PCD and pollen fertility. Our results reveal that CEP1 is a crucial executor during tapetal PCD and that proper CEP1 expression is necessary for timely degeneration of tapetal cells and functional pollen formation.

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“…All of the C1A proteases contain several disulfide bonds and share three conserved catalytic residues (Cys, His, and Asn) in the catalytic triad, a trait that is common to all Cysproteases, and they also contain a Gln involved in maintaining an active enzyme conformation. In addition, the GCNGG motif has been identified in all C1A protease members, and the noncontiguous ERFNIN motif has been found in cathepsin L-and H-like proteins (Grudkowska and Zagdanska, 2004;Zhang et al, 2009). C1A Cys-proteases from plants are synthesized as preproteins, processed either automatically or with the aid of processing enzymes, transported via the trans-Golgi network, and finally either are stored in the vacuoles and lysosomes or externally secreted (Grudkowska and Zagdanska, 2004).…”

Section: ([Lvi]-[agt]-[rke]-[fy]-[as]-[vi]-x-[edqv]-mentioning

confidence: 99%

Characterization of the Entire Cystatin Gene Family in Barley and Their Target Cathepsin L-Like Cysteine-Proteases, Partners in the Hordein Mobilization during Seed Germination

et al. 2009

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Plant cystatins are inhibitors of cysteine-proteases of the papain C1A and legumain C13 families. Cystatin data from multiple plant species have suggested that these inhibitors act as defense proteins against pests and pathogens and as regulators of protein turnover. In this study, we characterize the entire cystatin gene family from barley (Hordeum vulgare), which contain 13 nonredundant genes, and identify and characterize their target enzymes, the barley cathepsin L-like proteases. Cystatins and proteases were expressed and purified from Escherichia coli cultures. Each cystatin was found to have different inhibitory capability against barley cysteine-proteases in in vitro inhibitory assays using specific substrates. Real-time reverse transcriptionpolymerase chain reaction revealed that inhibitors and enzymes present a wide variation in their messenger RNA expression patterns. Their transcripts were mainly detected in developing and germinating seeds, and some of them were also expressed in leaves and roots. Subcellular localization of cystatins and cathepsin L-like proteases fused to green fluorescent protein demonstrated the presence of both protein families throughout the endoplasmic reticulum and the Golgi complex. Proteases and cystatins not only colocalized but also interacted in vivo in the plant cell, as revealed by bimolecular fluorescence complementation. The functional relationship between cystatins and cathepsin L-like proteases was inferred from their common implication as counterparts of mobilization of storage proteins upon barley seed germination. The opposite pattern of transcription expression in gibberellin-treated aleurones presented by inhibitors and enzymes allowed proteases to specifically degrade B, C, and D hordeins stored in the endosperm of barley seeds.

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NtCP56, a new cysteine protease in Nicotiana tabacum L., involved in pollen grain development

Cited by 34 publications

References 41 publications

Isolation of cDNA from Jacaratia mexicana encoding a mexicain-like cysteine protease gene

Isolation of cDNA from Jacaratia mexicana encoding a mexicain-like cysteine protease gene

The Cysteine Protease CEP1, a Key Executor Involved in Tapetal Programmed Cell Death, Regulates Pollen Development in Arabidopsis

Characterization of the Entire Cystatin Gene Family in Barley and Their Target Cathepsin L-Like Cysteine-Proteases, Partners in the Hordein Mobilization during Seed Germination

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