Analysis of the vacuolar luminal proteome of <i>Saccharomyces cerevisiae</i>

Sarry, Jean-Emmanuel; Chen, Sixue; Collum, Richard P.; Liang, Shun; Peng, Mingsheng; Lang, A.; Naumann, Bianca; Dzierszinski, Florence; Yuan, Chao‐Xing; Hippler, Michael; Rea, Philip A.

doi:10.1111/j.1742-4658.2007.05959.x

Cited by 36 publications

(43 citation statements)

References 67 publications

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“…Although most proteomics studies of multicellular organisms tend to use intact organs and tissues that contain many different cells, proteomics of individual cell types or organelles has become increasingly important because it allows fine dissection of cellular or organelle functions (45)(46)(47). Although the guard cell isolation procedure is tedious and the yield is relatively low, obtaining proteomics quality and quantity material is not limiting.…”

Section: Discussionmentioning

confidence: 99%

Functional Differentiation of Brassica napus Guard Cells and Mesophyll Cells Revealed by Comparative Proteomics

Zhu

Dai

McClung

et al. 2009

Molecular & Cellular Proteomics

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Guard cells (GC)1 are highly specialized cells that form tiny pores called stomata on the leaf surface. When environmental conditions change, guard cells can rapidly change shape so that the pores open or close to control leaf gas exchange and water transpiration. Mesophyll cells (MC) are mainly parenchyma cells between the upper and lower epidermis specialized for photosynthesis. Previous studies that focused on guard cell metabolism and response to environmental signals have revealed important features of functional differentiation of GC (1, 2). Compared with MC, GC contain few chloroplasts with very limited structures and thus possess very low photosynthetic capability. The Calvin cycle in GC only assimilates 2-4% of CO 2 fixed in MC (3). In contrast, GC contain abundant mitochondria and display a high respiratory rate, suggesting that oxidative phosphorylation is an important source of ATP to fuel the guard cell machinery (4). Using microarrays covering just one-third of the Arabidopsis genome, Leonhardt et al. (5) observed a differential abscisic acid (ABA) modulation of many guard cell ABA signaling components as well as key enzymes involved in carbon metabolism in GC and MC. This only available large scale genomics study identified 1309 guard cell expressed genes of which 64 transcripts mainly involved in transcription, signaling, and cytoskeleton were preferentially expressed in GC compared with MC. However, functional grouping of the genes revealed only a 1.9% higher representation of photosynthesis genes in MC than in GC. The percentages of genes in all other categories such as protein turnover, defense, signaling, channels and transporters, and metabolism are similar between the two distinct cell types (5). These proteins are known to play specific roles in guard cell functions (6). This highlights the necessity of studying guard cell functions at the protein level.To date, there have been very few analyses of single celltype proteomes in plants. Proteome analyses of trichomes from Arabidopsis (7) and tobacco (8) and root hairs from soybean (9) exist but have identified fewer than 100 proteins per proteome. The proteomes of pollen from different species have been relatively well studied, but the pollen grains are not single cells because they contain two/three-cell gametophytes (10). A critical factor for large scale proteomics analFrom the ‡Department

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Section: Discussionmentioning

confidence: 99%

Functional Differentiation of Brassica napus Guard Cells and Mesophyll Cells Revealed by Comparative Proteomics

Zhu

Dai

McClung

et al. 2009

Molecular & Cellular Proteomics

Self Cite

111

115

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“…The mitochondrial marker succinate dehydrogenase was assayed by quantifying reduced p-iodonitrotetrazolium violet 48,51 . Finally, carboxypeptidase Y and a-D-mannosidase were employed as markers for the vacuolar lumen and membrane, respectively 28,52,53 . Carboxypeptidase Y activity was based on the release of leucine from N-CBZ-L-Phe-L-Leu.…”

Section: Methodsmentioning

confidence: 99%

Caesium accumulation in yeast and plants is selectively repressed by loss of the SNARE Sec22p/SEC22

Dräxl

Müller

et al. 2013

Nat Commun

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The non-essential cation caesium (Cs þ ) is assimilated by all organisms. Thus, anthropogenically released radiocaesium is of concern to agriculture. Cs þ accumulates owing to its chemical similarity to the potassium ion (K þ ). The apparent lack of a Cs þ -specific uptake mechanism has obstructed attempts to manipulate Cs þ accumulation without causing pleiotropic effects. Here we show that the SNARE protein Sec22p/SEC22 specifically impacts Cs þ accumulation in yeast and in plants. Loss of Saccharomyces cerevisiae Sec22p does not affect K þ homeostasis, yet halves Cs þ concentration compared with the wild type. Mathematical modelling of the uptake time course predicts a compromised vacuolar Cs þ deposition in sec22D. Biochemical fractionation confirms this and indicates a new feature of Sec22p in enhancing non-selective cation deposition. A developmentally controlled loss-of-function mutant of the orthologous Arabidopsis thaliana SEC22 phenocopies the reduced Cs þ uptake without affecting plant growth. This finding provides a new strategy to reduce radiocaesium entry into the food chain.

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“…The integrity of the vacuoles prepared in this way was assessed by testing their ability to retain the fluorescent glutathione S-conjugate of monochlorobimane (MCB), bimane-GS (6,21). MCB is a membrane-permeant, non-fluorescent compound that is specifically conjugated with GSH by cytosolic glutathione S-transferases to generate the intensely fluorescent, membrane-impermeant product bimane-GS that is actively transported into and sequestered within the vacuole of intact cells.…”

Section: Assessment Of Integrity Of Vacuole Preparations-mentioning

confidence: 99%

Drosophila ABC Transporter, DmHMT-1, Confers Tolerance to Cadmium

Sooksa-nguan

Yakubov

Kozlovskyy

et al. 2009

Journal of Biological Chemistry

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Half-molecule ATP-binding cassette transporters of the HMT-1 (heavy metal tolerance factor 1) subfamily are required for Cd 2؉ tolerance in Schizosaccharomyces pombe, Caenorhabditis elegans, and Chlamydomonas reinhardtii. Based on studies of S. pombe, it has been proposed that SpHMT-1 transports heavy metal⅐phytochelatin (PC) complexes into the vacuolysosomal compartment. PCs are glutathione derivatives synthesized by PC synthases (PCS) in plants, fungi, and C. elegans in response to heavy metals. Our previous studies in C. elegans, however, suggested that HMT-1 and PCS-1 do not necessarily act in concert in metal detoxification. To further explore this inconsistency, we have gone on to test whether DmHMT-1, an HMT-1 from a new source, Drosophila, whose genome lacks PCS homologs, functions in heavy metal detoxification. In so doing, we show that heterologously expressed DmHMT-1 suppresses the Cd 2؉ hypersensitivity of S. pombe hmt-1 mutants and localizes to the vacuolar membrane but does not transport Cd⅐PC complexes. Crucially, similar analyses of S. pombe hmt-1 mutants extend this finding to show that SpHMT-1 itself either does not transport Cd⅐PC complexes or is not the principal Cd⅐PC/apoPC transporter. Consistent with this discovery and with our previous suggestion that HMT-1 and PCS-1 do not operate in a simple linear metal detoxification pathway, we demonstrate that, unlike PCS-deficient cells, which are hypersensitive to several heavy metals, SpHMT-1-deficient cells are hypersensitive to Cd 2؉ , but not to Hg 2؉ or As 3؉ . These findings significantly change our current understanding of the function of HMT-1 proteins and invoke a PC-independent role for these transporters in Cd 2؉ detoxification.The adverse health effects of heavy metals such as cadmium (Cd 2ϩ ), mercury (Hg 2ϩ ), and lead (Pb 2ϩ ) from food and air are well established (1-4). Despite this knowledge, exposure to heavy metals continues, and has even increased in some areas, due to their sustained production and emission into the environment. At the cellular level, the toxicity of heavy metals results from the displacement of endogenous cofactors from their cellular binding sites, the oxidation of essential enzymes and other proteins, and promotion of the formation of reactive oxygen species (3, 4). The variety of ways by which heavy metals exert their effects places demands on a wide range of distinct cellular detoxification mechanisms in which ATP-binding cassette (ABC) 3 transporters are clearly implicated (5-9). The ABC transporter family is one of the largest families of membrane proteins. Although 60 ABC transporter family members are known in Caenorhabditis elegans, 49 in humans, 57 in Drosophila, 103 in Arabidopsis, 30 in Saccharomyces cerevisiae, and 11 in Schizosaccharomyces pombe (10 -13), the exact role played by the many that are implicated in heavy metal detoxification remains to be determined. What is known is that ABC transporters mediate the Mg⅐ATP-energized transmembrane transport of a wide range of substrates, reside on ...

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Analysis of the vacuolar luminal proteome of Saccharomyces cerevisiae

Cited by 36 publications

References 67 publications

Functional Differentiation of Brassica napus Guard Cells and Mesophyll Cells Revealed by Comparative Proteomics

Functional Differentiation of Brassica napus Guard Cells and Mesophyll Cells Revealed by Comparative Proteomics

Caesium accumulation in yeast and plants is selectively repressed by loss of the SNARE Sec22p/SEC22

Drosophila ABC Transporter, DmHMT-1, Confers Tolerance to Cadmium

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