Influence of ryanodine on the mechanical restitution and on the post-extrasystolic potentiation of the guinea-pig ventricular myocardium

This paper records the results of an investigation into potentiation and staircase phenomena in rightventricular guinea-pig papillary muscles with particular reference to the sarcoplasmic Ca²⁺-channel. As a tool to isolate the second (late, 1tonic) component of isoproterenol-induced biphasic contractions ryanodine was used. On the evidence at present available the monophasic ryanodine-resistant component of the twitch represents that portion of the activator calcium which reaches the troponin C directly, that is, not taking the roundabout way through the intracellular storage structures. In order to avoid functional instabilities of the isolated muscle preparation a short-time double rest stimulation programme was used which combines a number of different tests and gives information on (1) the post-rest potentiation, (2) the post-extrasystolic potentiation, (3) the mechanical post-rest recovery, (4) the interval-strength relationship, and (5) the mechanical restitution. The results of the present work show that under the influence of ryanodine (1) the BOWDITCH staircase, a typical feature of normodynamic mammalian ventricular preparations as well as of hypodynamic frog heart preparations, does not exist, (2) the post-extrasystolic potentiation disappears, (3) the curve reflecting the mechanical restitution, under normal in vitro conditions a monotonically increasing function, becomes biphasic within the relative refractory period, (4) the conspicuous depression of the isometric post-rest contraction for long iasting pauses interrupting the regular pacing rhythm, a typical feature of isolated guinea-pig ventricular tissue, is clearly diminished, and (5) the characteristic curve, reflecting the potentiation of the post-extrasystolic post-rest contraction as a function of the delay time preceding the extrastimulus, becomes displaced to the premature interstimulus interval. The concept of an extended 2-calcium-store model is supported by this work.     

Leadzyme formed in vivo interferes with tobacco mosaic virus infection in Nicotiana tabacum

We developed a new method for inhibiting tobacco mosaic virus infection in tobacco plants based on specific RNA hydrolysis induced by a leadzyme. We identified a leadzyme substrate target sequence in genomic tobacco mosaic virus RNA and designed a 16-mer oligoribonucleotide capable of forming a specific leadzyme motif with a five-nucleotide catalytic loop. The synthetic 16-mer RNA was applied with nontoxic, catalytic amount of lead to infected tobacco leaves. We observed inhibition of tobacco mosaic virus infection in tobacco leaves in vivo due to specific tobacco mosaic virus RNA cleavage effected by leadzyme. A significant reduction in tobacco mosaic virus accumulation was observed even when the leadzyme was applied up to 2 h after inoculation of leaves with tobacco mosaic virus. This process, called leadzyme interference, is determined by specific recognition and cleavage of the target site by the RNA catalytic strand in the presence of Pb(2+).     

Biosynthesis of the N-linked glycan in Campylobacter jejuni and addition onto protein through block transfer

In eukaryotes, N-linked protein glycosylation is a universal modification involving addition of preformed oligosaccharides to select Asn-Xaa-Ser/Thr motifs and influencing multiple biological events. We recently demonstrated that Campylobacter jejuni is the first member of the Bacteria to possess an N-linked glycan pathway. In this study, high-resolution magic angle spinning nuclear magnetic resonance (HR-MAS NMR) was applied to probe and quantitate C. jejuni N-glycan biosynthesis in vivo. To confirm HR-MAS NMR findings, glycosylation mutants were screened for chicken colonization potential, and glycoproteins were examined by mass spectrometry and lectin blotting. Consistent with the mechanism in eukaryotes, the combined data indicate that bacterial glycans are assembled en bloc, emphasizing the evolutionary conservation of protein N glycosylation. We also show that under the conditions examined, PglG plays no role in glycan biosynthesis, PglI is the glucosyltransferase and the putative ABC transporter, and WlaB (renamed PglK) is required for glycan assembly. These studies underpin the mechanism of N-linked protein glycosylation in Bacteria and provide a simple model system for investigating protein glycosylation and for exploitation in glycoengineering.     

Modification of the Campylobacter jejuni N-Linked Glycan by EptC Protein-mediated Addition of Phosphoethanolamine

Campylobacter jejuni is the major worldwide cause of bacterial gastroenteritis. C. jejuni possesses an extensive repertoire of carbohydrate structures that decorate both protein and non-protein surface-exposed structures. An N-linked glycosylation system encoded by the pgl gene cluster mediates the synthesis of a rigidly conserved heptasaccharide that is attached to protein substrates or released as free oligosaccharide in the periplasm. Removal of N-glycosylation results in reduced virulence and impeded host cell attachment. Since the N-glycan is conserved, the N-glycosylation system is also an attractive option for glycoengineering recombinant vaccines in Escherichia coli. To determine whether non-canonical N-glycans are present in C. jejuni, we utilized high throughput glycoproteomics to characterize C. jejuni JHH1 and identified 93 glycosylation sites, including 34 not previously reported. Interrogation of these data allowed the identification of a phosphoethanolamine (pEtN)-modified variant of the N-glycan that was attached to multiple proteins. The pEtN moiety was attached to the terminal GalNAc of the canonical N-glycan. Deletion of the pEtN transferase eptC removed all evidence of the pEtN-glycan but did not globally influence protein reactivity to patient sera, whereas deletion of the pglB oligosaccharyltransferase significantly reduced reactivity. Transfer of eptC and the pgl gene cluster to E. coli confirmed the addition of the pEtN-glycan to a target C. jejuni protein. Significantly reduced, yet above background levels of pEtN-glycan were also observed in E. coli not expressing eptC, suggesting that endogenous E. coli pEtN transferases can mediate the addition of pEtN to N-glycans. The addition of pEtN must be considered in the context of glycoengineering and may alter C. jejuni glycan-mediated structure-function interactions.     

Unraveling Sterol-dependent Membrane Phenotypes by Analysis of Protein Abundance-ratio Distributions in Different Membrane Fractions Under Biochemical and Endogenous Sterol Depletion

During the last decade, research on plasma membrane focused increasingly on the analysis of so-called microdomains. It has been shown that function of many membrane-associated proteins involved in signaling and transport depends on their conditional segregation within sterol-enriched membrane domains. High throughput proteomic analysis of sterol-protein interactions are often based on analyzing detergent resistant membrane fraction enriched in sterols and associated proteins, which also contain proteins from these microdomain structures. Most studies so far focused exclusively on the characterization of detergent resistant membrane protein composition and abundances. This approach has received some criticism because of its unspecificity and many co-purifying proteins. In this study, by a label-free quantitation approach, we extended the characterization of membrane microdomains by particularly studying distributions of each protein between detergent resistant membrane and detergent-soluble fractions (DSF). This approach allows a more stringent definition of dynamic processes between different membrane phases and provides a means of identification of co-purifying proteins. We developed a random sampling algorithm, called Unicorn, allowing for robust statistical testing of alterations in the protein distribution ratios of the two different fractions. Unicorn was validated on proteomic data from methyl-β-cyclodextrin treated plasma membranes and the sterol biosynthesis mutant smt1. Both, chemical treatment and sterol-biosynthesis mutation affected similar protein classes in their membrane phase distribution and particularly proteins with signaling and transport functions.The plasma membrane incorporates a broad spectrum of proteins covering mainly different structural, signaling or transport functionalities. Being the first semipermeable cell barrier to its surrounding environment the plasma membrane is important for metabolite transport as well as initiation point of several signaling processes (1–4). To maintain cell homeostasis, protein activity as well as complex formation through protein protein interactions (PPI) need to be tightly regulated. The major regulating mechanisms are postranslational modification of proteins and modulated abundances of proteins present in the plasma membrane. Another potential regulating mechanism became apparent with the discovery of sterol and sphingolipid enriched domains (microdomains) in the plasma membrane (5–8, 3). Microdomain like structures have been shown to form spontaneously in artificial plasma membranes (9). After a decade of research on these structures, microdomains turned out to be particularly involved in signaling and transport processes incorporating a specific set of proteins. Microdomains provide subcompartments in the plasma membrane with specific physicochemical properties that on specific sterol protein interactions might alter protein activity or PPIs. With the discovery of microdomains the fluid lipid mosaic model was extended by distinguishing two plasma membrane phases, an ordered phase of lower density (L_o phase) enriched in sterols, sphingolipids and long chain fatty acids and a disordered phase of higher density (L_d phase). From isolated plasma membranes a lower density and a higher density membrane fraction can be separated in a sucrose gradient after treatment with non-ionic detergents. The resulting detergent resistant membrane fraction (DRM)¹ is related to L_o phase and high density detergent soluble membrane fraction (DSF) relates to L_o phases. Although it is still under debate how well DRMs represent native plasma membrane microdomains (10–12), research on protein-sterol interactions is possible by usage of sterol depleting agents like methyl-β-cyclodextrin mβcd (13). Therefore mβcd is suitable for detecting false positive cholesterol protein interactions in DRM studies (14–19). Proteins depleted on mβcd treatment are finally considered to be sterol dependent (15–17). To compare the mβcd treatment for disturbing the sterol distribution in the L_o fraction, we studied the sterol biosynthesis deficient mutant smt1. (20) smt1 carries a point mutation in the smt1 locus, encoding the sterol methyltransferase 1 and it exhibits a dwarf-like phenotype on whole plant level (20). In total, three sterol methyl transferases are encoded in Arabidopsis where SMT1 catalyzes the first step in the sterol biosynthesis by adding a methyl group at C24 of the sterol precursor cycloartenol. SMT2 and SMT3 act at later steps and were shown to be functionally redundant as C-24 sterol methyltransferases at the branching in sterol synthesis that either leads to sitosterol or campesterol (21). The total sterol composition in smt1 mutants was shown to be different from wild type, with the major phytosterols like sitosterol, stigmasterol, and brassicasterol being strongly depleted. In contrast, other sterol species remained unaltered and some even increased (20, 21). So far, it remains unclear how the altered sterol-composition of the smt1 mutant affects sterol-protein interactions. In this study, using the newly developed algorithm Unicorn, we compared changes in protein distributions between DRM and DSF after biochemical mβcd treatment and on endogenous alterations in sterol composition in smt1 to improve understanding of sterol–protein interactions.     

Development of novel molecular probes of the Rio1 atypical protein kinase

The RIO kinases are essential protein factors required for the synthesis of new ribosomes in eukaryotes. Conserved in archaeal organisms as well, RIO kinases are among the most ancient of protein kinases. Their exact molecular mechanisms are under investigation and progress of this research would be significantly improved with the availability of suitable molecular probes that selectively block RIO kinases. RIO kinases contain a canonical eukaryotic protein kinase fold, but also display several unusual structural features that potentially create opportunity for the design of selective inhibitors. In an attempt to identify structural leads to target the RIO kinases, a series of pyridine caffeic acid benzyl amides (CABA) were tested for their ability to inhibit the autophosphorylation activity of Archeaoglobus fulgidus Rio1 (AfRio1). Screening of a small library of CABA molecules resulted in the identification of four compounds that measurably inhibited AfRio1 activity. Additional biochemical characterization of binding and inhibition activity of these compounds demonstrated an ATP competitive inhibition mode, and allowed identification of the functional groups that result in the highest binding affinity. In addition, docking of the compound to the structure of Rio1 and determination of the X-ray crystal structure of a model compound (WP1086) containing the desired functional groups allowed detailed analysis of the interactions between these compounds and the enzyme. Furthermore, the X-ray crystal structure demonstrated that these compounds stabilize an inactive form of the enzyme. Taken together, these results provide an important step in identification of a scaffold for the design of selective molecular probes to study molecular mechanisms of Rio1 kinases in vitro and in vivo. In addition, it provides a rationale for the future design of potent inhibitors with drug-like properties targeting an inactive form of the enzyme. This article is part of a Special Issue entitled: Inhibitors of Protein Kinases (2012).     

The Endoplasmic Reticulum Is a Reservoir for WAVE/SCAR Regulatory Complex Signaling in the Arabidopsis Leaf

During plant cell morphogenesis, signal transduction and cytoskeletal dynamics interact to locally organize the cytoplasm and define the geometry of cell expansion. The WAVE/SCAR (for WASP family verprolin homologous/suppressor of cyclic AMP receptor) regulatory complex (W/SRC) is an evolutionarily conserved heteromeric protein complex. Within the plant kingdom W/SRC is a broadly used effector that converts Rho-of-Plants (ROP)/Rac small GTPase signals into Actin-Related Protein2/3 and actin-dependent growth responses. Although the components and biochemistry of the W/SRC pathway are well understood, a basic understanding of how cells partition W/SRC into active and inactive pools is lacking. In this paper, we report that the endoplasmic reticulum (ER) is an important organelle for W/SRC regulation. We determined that a large intracellular pool of the core W/SRC subunit NAP1, like the known positive regulator of W/SRC, the DOCK family guanine nucleotide-exchange factor SPIKE1 (SPK1), localizes to the surface of the ER. The ER-associated NAP1 is inactive because it displays little colocalization with the actin network, and ER localization requires neither activating signals from SPK1 nor a physical association with its W/SRC-binding partner, SRA1. Our results indicate that in Arabidopsis (Arabidopsis thaliana) leaf pavement cells and trichomes, the ER is a reservoir for W/SRC signaling and may have a key role in the early steps of W/SRC assembly and/or activation.The W/SRC (for WASP family verprolin homologous/suppressor of cAMP receptor regulatory complex) and Actin-Related Protein (ARP)2/3 complex are part of an evolutionarily conserved Rho-of-Plants (ROP)/Rac small GTPase signal transduction cascade that controls actin-dependent morphogenesis in a wide variety of tissues and developmental contexts (Smith and Oppenheimer, 2005; Szymanski, 2005; Yalovsky et al., 2008). Many of the components and regulatory relationships among the complexes were discovered based on the stage-specific cell-swelling and -twisting phenotypes of the distorted class of Arabidopsis (Arabidopsis thaliana) trichome mutants (Szymanski et al., 1999; Zhang et al., 2005, 2008; Djakovic et al., 2006; Le et al., 2006; Uhrig et al., 2007). However, in both maize (Zea mays) and Arabidopsis, W/SRC and/or ARP2/3 are required for normal pavement cell morphogenesis (Frank and Smith, 2002; Mathur et al., 2003b; Brembu et al., 2004). Compared with other Arabidopsis pavement cell mutants, the shape defects of the distorted group are relatively mild. However, the distorted mutants and spike1 (spk1) differ from most other morphology mutants in that they display gaps in the shoot epidermis, most frequently at the interface of pavement cells and stomata (Qiu et al., 2002; Le et al., 2003; Li et al., 2003; Mathur et al., 2003b; Zhang et al., 2005; Djakovic et al., 2006). The cell gaps may reflect either uncoordinated growth between neighboring cells or defective cortical actin-dependent secretion of polysaccharides and/or proteins that promote cell-cell adhesion (Smith and Oppenheimer, 2005; Hussey et al., 2006; Leucci et al., 2007).In tip-growing cells, there is a strict requirement for actin to organize the trafficking and secretion activities of the cell to restrict growth to the apex. In Arabidopsis, the W/SRC-ARP2/3 pathway is not an essential tip growth component, because null alleles of both W/SRC and ARP2/3 subunits do not cause noticeable pollen tube or root hair phenotypes (Le et al., 2003; Djakovic et al., 2006). However, reverse genetic analysis of the W/SRC subunit BRK1 and ARP2/3 in the tip-growing protonemal cells of Physcomitrella patens revealed the obvious importance of this pathway (Harries et al., 2005; Perroud and Quatrano, 2008). Along similar lines, in two different legume species, W/SRC subunits are required for a normal root nodulation response to symbiotic bacteria (Yokota et al., 2009; Miyahara et al., 2010), indicating a conditional importance for this pathway in root hair growth. These genetic studies centered on the W/SRC and ARP2/3 pathways, in addition to those that involve a broader collection of actin-based morphology mutants (Smith and Oppenheimer, 2005; Blanchoin et al., 2010), are defining important cytoskeletal proteins and new interactions with the endomembrane system during morphogenesis. However, it is not completely clear how unstable actin filaments and actin bundle networks dictate the growth patterns of cells (Staiger et al., 2009).The difficulty of understanding the functions of specific actin arrays can be explained, in part, by the fact that plant cells that employ a diffuse growth mechanism have highly unstable cortical actin filaments and large actin bundles that do not have a geometry that obviously relates to the direction of growth or a specific subcellular activity (Blanchoin et al., 2010). This is in contrast to the cortical endocytic actin patches in yeast (Saccharomyces cerevisiae; Evangelista et al., 2002; Kaksonen et al., 2003) and cortical meshworks in the lamellipodia of crawling cells (Pollard and Borisy, 2003) that reveal subcellular locations where actin works to locally control membrane dynamics. In thick-walled plant cells, the magnitude of the forces that accompany turgor-driven cell expansion exceed those that could be generated by actin polymerization by orders of magnitude (Szymanski and Cosgrove, 2009). Localized cell wall loosening or the assembly of an anisotropic cell wall generates asymmetric yielding responses to turgor-induced stress (Baskin, 2005; Cosgrove, 2005). Therefore, the actin-based control of cell boundary dynamics is indirect, and the actin cytoskeleton influences cell shape change, in part, by actin and/or myosin-dependent trafficking of hormone transporters (Geldner et al., 2001) and organelles (Prokhnevsky et al., 2008), including those that control the localized delivery of protein complexes and polysaccharides that pattern the cell wall (Leucci et al., 2007; Gutierrez et al., 2009). In this scheme for actin-based growth control, the actin network dynamically rearranges at spatial scales that span from approximately 1- to 10-µm subcellular domains that may locally position organelles (Cleary, 1995; Gibbon et al., 1999; Szymanski et al., 1999) to the more than 100-µm actin bundle networks that operate at the spatial scales of entire cells (Gutierrez et al., 2009; Dyachok et al., 2011). It is clear from the work of several laboratories that the W/SRC and ARP2/3 protein complexes are required to organize cortical actin and actin bundle networks in trichomes (Szymanski et al., 1999; Le et al., 2003; Deeks et al., 2004; Zhang et al., 2005) and cylindrical epidermal cells (Mathur et al., 2003b; Dyachok et al., 2008, 2011). A key challenge now is to understand how plant cells deploy these approximately 10- to 20-nm heteromeric protein complexes to influence the patterns of growth at cellular scales.The genetic and biochemical control of ARP2/3 is complicated, but this is a tractable problem in plants, because the pathway is relatively simple compared with most other species in which it has been characterized. For example, in organisms ranging from yeast to humans, there are multiple types of ARP2/3 activators, protein complexes, and pathways that activate ARP2/3 (Welch and Mullins, 2002; Derivery and Gautreau, 2010). However, the maize and Arabidopsis genomes encode only WAVE/SCAR homologous proteins that can potently activate ARP2/3 (Frank et al., 2004; Basu et al., 2005). Detailed genetic and biochemical analyses of the WAVE/SCAR gene family in Arabidopsis demonstrated that the plant activators function interchangeably within the context of the W/SRC and define the lone pathway for ARP2/3 activation (Zhang et al., 2008). Bioinformatic analyses are consistent with a prominent role for W/SRC in the angiosperms, because in general, WASH complex subunits, which are structurally similar to WAVE/SCAR proteins, are largely absent from the higher plant genomes, while WAVE/SCAR genes are highly conserved (Kollmar et al., 2012).The components and regulatory schemes of the W/SRC-ARP2/3 pathway in Arabidopsis and P. patens are conserved compared with vertebrate species that employ these same protein complexes (Szymanski, 2005). For example, mutant complementation tests indicate that human W/SRC and ARP2/3 complex subunits can substitute for the Arabidopsis proteins (Mathur et al., 2003b). Furthermore, biochemical assays of Arabidopsis W/SRC (Basu et al., 2004; El-Assal et al., 2004; Frank et al., 2004; Le et al., 2006; Uhrig et al., 2007) and ARP2/3 assembly (Kotchoni et al., 2009) have shown that the binary interactions among W/SRC subunits and ARP2/3 complex assembly mechanisms are indistinguishable from those that have been observed for human W/SRC (Gautreau et al., 2004) and yeast ARP2/3 (Winter et al., 1999). After an initial period of controversy concerning the biochemical control of W/SRC, it is now apparent that vertebrate W/SRC (Derivery et al., 2009; Ismail et al., 2009), like the ARP2/3 complex (Machesky et al., 1999), is intrinsically inactive and requires positive regulation by Rac and other factors to fully activate ARP2/3 (Ismail et al., 2009; Lebensohn and Kirschner, 2009; Chen et al., 2010). Although overexpression of dominant negative ROP mutants causes trichome swelling and a reduced trichome branch number (Fu et al., 2002), the involvement of ROPs in trichome morphogenesis has been difficult to prove with a loss-of-function ROP allele because so many ROPs are expressed in this cell type (Marks et al., 2009). Existing reports on ROP loss-of-function mutants demonstrate the importance of pavement cell morphogenesis but do not document a trichome phenotype (Fu et al., 2005; Xu et al., 2010). A recent report describes a clever strategy to generate ROP loss-of-function lines that used the ectopic expression of ROP-specific bacterial toxins. There was a strong association between inducible expression of the toxins and the appearance of trichomes with severe trichome swelling and reduced branch number phenotypes (Singh et al., 2012). Although the exact mechanism of ROP-dependent control of W/SRC remains to be determined, the results described above in combination with the detection of direct interactions between the ROPGEF SPK1, active forms of ROP, and W/SRC subunits (Basu et al., 2004, 2008; Uhrig et al., 2007) strongly suggest that W/SRC is a ROP effector complex.The major challenge in the field now is to better understand the cellular control of W/SRC and how the complex is partitioned into active and inactive pools. In mammalian cells that crawl on a solid substrate, current models propose that a cytosolic pool of inactive WAVE/SCAR proteins and W/SRC is locally recruited and activated at specific plasma membrane surfaces in response to signals from some unknown Rac guanine nucleotide-exchange factor (GEF), protein kinase, and/or lipid kinase (Oikawa et al., 2004; Lebensohn and Kirschner, 2009; Chen et al., 2010). However, in Drosophila melanogaster neurons (Bogdan and Klämbt, 2003) and cultured human melanoma cells (Steffen et al., 2004), there are large pools of W/SRC with a perinuclear or organelle-like punctate localization that has no obvious relationship to cell shape or motility, raising uncertainty about the cellular mechanisms of W/SRC activation and the importance of different subcellular pools of the complex.In plants, cell fractionation experiments indicate that SCAR1 and ARP2/3 have an increased association with membranes compared with their animal counterparts (Dyachok et al., 2008; Kotchoni et al., 2009). In tip-growing moss protonemal cells, both the W/SRC subunit BRK1 and ARP2/3 localize to a population of unidentified organelles within the apical zone (Perroud and Quatrano, 2008). Similar live-cell imaging experiments in Arabidopsis reported a plasma membrane localization for SCAR1 and BRK1 in a variety of shoot epidermal and root cortex, and their accumulation at young trichome branch tips and at three-way cell wall junctions may define subcellular domains for W/SRC-ARP2/3-dependent actin filament nucleation at the plasma membrane (Dyachok et al., 2008). However, to our knowledge, active W/SRC, defined here as the fraction of W/SRC that colocalizes with ARP2/3 or actin, has not been reported in plants, and the plasma membrane is not necessarily the only organelle involved in W/SRC regulation. For example, the reported accumulation of BRK1 and SCAR1 at three-way cell wall junctions has a punctate appearance at the cell cortex that may not simply correspond to the plasma membrane (Dyachok et al., 2008). Also, in young stage 4 trichomes, there was an uncharacterized pool of intracellular SCAR1, but not BRK1, that localized to relatively large punctate structures (Dyachok et al., 2008). The endoplasmic reticulum (ER) may also be involved in W/SRC regulation. The ER-localized DOCK family ROPGEF SPK1 (Zhang et al., 2010) physically associates with multiple W/SRC proteins (Uhrig et al., 2007; Basu et al., 2008) and, based on genetic criteria, is an upstream, positive regulator of the W/SRC-ARP2/3 pathway (Basu et al., 2008). In the leaf, one function of SPK1 is to promote normal trafficking between the ER and Golgi; however, arp2/3 mutants do not share ER-stress phenotypes with spk1 (Zhang et al., 2010), making it unclear if SPK1 and the ER are directly involved in W/SRC signaling.This paper focuses on the localization and control of the W/SRC subunit NAP1/GNARLED/NAPP/HEM1/2. Arabidopsis NAP1 directly interacts with the ROP/Rac effector subunit SRA1/PIROGI/KLUNKER/PIRP (Basu et al., 2004; El-Assal et al., 2004; Uhrig et al., 2007). Based on the equally severe syndrome of nap1 and arp2/3 null phenotypes, and double mutant analyses, the only known function of NAP1 is to positively regulate ARP2/3 (Brembu et al., 2004; Deeks et al., 2004; El-Din El-Assal et al., 2004; Li et al., 2004). The vertebrate SRA1-NAP1 dimer is important for W/SRC assembly (Gautreau et al., 2004) and forms an extended physical surface that trans-inhibits the C-terminal ARP2/3-activating domain of WAVE/SCAR (Chen et al., 2010). The plant NAP1 and SRA1 proteins share end-to-end amino acid conservation with their vertebrate homologs and may form a heterodimer with similar functions (Basu et al., 2004; El-Assal et al., 2004; Uhrig et al., 2007). We report here that Arabidopsis NAP1 is strongly associated with ER membranes. In a detailed series of localization experiments, we detect a complicated intracellular distribution of NAP1 among the ER, the nucleus, and unidentified submicrometer punctae. A large pool of ER-associated NAP1 is inactive, based on the low level of colocalization with actin.Its accumulation on the ER does not require activating signals from either SPK1 or SRA1. These data indicate that the ER is a reservoir for W/SRC signaling and suggest that early steps in the positive regulation of NAP1 and the W/SRC occur on the ER surface.     

Analysis of short-term changes in the Arabidopsis thaliana glycerolipidome in response to temperature and light

Although the influence of temperature, particularly cold, on lipid metabolism is well established, previous studies have focused on long-term responses and have largely ignored the influence of other interacting environmental factors. Here, we present a time-resolved analysis of the early responses of the glycerolipidome of Arabidopsis thaliana plants exposed to various temperatures (4, 21 and 32°C) and light intensities (darkness, 75, 150 and 400 μmol m(-2) s(-1)), including selected combinations. Using a UPLC/MS-based lipidomic platform, we reproducibly measured most glycerolipid species reported for Arabidopsis leaves, including the classes phosphatidylcholine (PC), phosphatidylethanolamine (PE), phosphatidylserine (PS), phosphatidylinositol (PI) phosphatidylglycerol (PG), monogalactosyldiacylglycerol (MGDG), digalactosyldiacylglycerol (DGDG) and sulfoquinovosyldiacylglycerol (SQDG). In addition to known lipids, we have identified previously unobserved compounds, such as 36-C PGs and eukaryotic phospholipids containing 16:3 acyl chains. Occurrence of these lipid species implies the action of new biochemical mechanisms. Exposition of Arabidopsis plants to various light and temperature regimes results in two major effects. The first is the dependence of the saturation level of PC and MGDG pools on light intensity, likely arising from light regulation of de novo fatty acid synthesis. The second concerns an immediate decrease in unsaturated species of PG at high-temperature conditions (32°C), which could mark the first stages of adaptation to heat-stress conditions. Observed changes are discussed in the context of current knowledge, and new hypotheses have been formulated concerning the early stages of the plant response to changing light and temperature conditions.     

Metabolic Labeling and Membrane Fractionation for Comparative Proteomic Analysis of Arabidopsis thaliana Suspension Cell Cultures

Plasma membrane microdomains are features based on the physical properties of the lipid and sterol environment and have particular roles in signaling processes. Extracting sterol-enriched membrane microdomains from plant cells for proteomic analysis is a difficult task mainly due to multiple preparation steps and sources for contaminations from other cellular compartments. The plasma membrane constitutes only about 5-20% of all the membranes in a plant cell, and therefore isolation of highly purified plasma membrane fraction is challenging. A frequently used method involves aqueous two-phase partitioning in polyethylene glycol and dextran, which yields plasma membrane vesicles with a purity of 95% ¹. Sterol-rich membrane microdomains within the plasma membrane are insoluble upon treatment with cold nonionic detergents at alkaline pH. This detergent-resistant membrane fraction can be separated from the bulk plasma membrane by ultracentrifugation in a sucrose gradient ². Subsequently, proteins can be extracted from the low density band of the sucrose gradient by methanol/chloroform precipitation. Extracted protein will then be trypsin digested, desalted and finally analyzed by LC-MS/MS. Our extraction protocol for sterol-rich microdomains is optimized for the preparation of clean detergent-resistant membrane fractions from Arabidopsis thaliana cell cultures.We use full metabolic labeling of Arabidopsis thaliana suspension cell cultures with K¹⁵NO₃ as the only nitrogen source for quantitative comparative proteomic studies following biological treatment of interest ³. By mixing equal ratios of labeled and unlabeled cell cultures for joint protein extraction the influence of preparation steps on final quantitative result is kept at a minimum. Also loss of material during extraction will affect both control and treatment samples in the same way, and therefore the ratio of light and heave peptide will remain constant. In the proposed method either labeled or unlabeled cell culture undergoes a biological treatment, while the other serves as control ⁴.