Stabilization of the H,K-ATPase M5M6 membrane hairpin by K+ ions. Mechanistic significance for p2-type atpases.

The integral membrane protein, the gastric H,K-ATPase, is an alpha-beta heterodimer, with 10 putative transmembrane segments in the alpha-subunit and one such segment in the beta-subunit. All transmembrane segments remain within the membrane domain following trypsinization of the intact gastric H,K-ATPase in the presence of K+ ions, identified as M1M2, M3M4, M5M6, and M7, M8, M9, and M10. Removal of K+ ions from this digested preparation results in the selective loss of the M5M6 hairpin from the membrane. The release of the M5M6 fragment is directed to the extracellular phase as evidenced by the accumulation of the released M5M6 hairpin inside the sealed inside out vesicles. The stabilization of the M5M6 hairpin in the membrane phase by the transported cation as well as loss to the aqueous phase in the absence of the transported cation has been previously observed for another P2-type ATPase, the Na, K-ATPase (Lutsenko, S., Anderko, R., and Kaplan, J. H. (1995) Proc. Natl. Acad. Sci. U. S. A. 92, 7936-7940). Thus, the effects of the counter-transported cation on retention of the M5M6 segment in the membrane as compared with the other membrane pairs may be a general feature of P2-ATPase ion pumps, reflecting a flexibility of this region that relates to the mechanism of transport.     

Cys(577) is a conformationally mobile residue in the ATP-binding domain of the Na,K-ATPase alpha-subunit.

2-[4'-Maleimidylanilino]naphthalene 6-sulfonic acid (MIANS) irreversibly inactivates Na,K-ATPase in a time- and concentration-dependent manner. Inactivation is prevented by 3 mM ATP or low K(+) (<1 mM); the protective effect K(+) is reversed at higher concentrations. This biphasic effect was also observed with K(+) congeners. In contrast, Na(+) ions did not protect. MIANS inactivation disrupted high affinity ATP binding. Tryptic fragments of MIANS-labeled protein were analyzed by reversed phase high performance liquid chromatography. ATP clearly protected one major labeled peptide peak. This observation was confirmed by separation of tryptic peptides in SDS-polyacrylamide gel electrophoresis revealing a single fluorescently-labeled peptide of approximately 5 kDa. N-terminal amino acid sequencing identified the peptide (V(545)LGFCH...). This hydrophobic peptide contains only two Cys residues in all sodium pump alpha-subunit sequences and is found in the major cytoplasmic loop between M4 and M5, a region previously associated with ATP binding. Subsequent digestion of the tryptic peptide with V8 protease and N-terminal amino acid sequencing identified the modified residue as Cys(577). The cation-dependent change in reactivity of Cys(577) implies structural alterations in the ATP-binding domain following cation binding and occlusion in the intramembrane domain of Na,K-ATPase and expands our knowledge of the extent to which cation binding and occlusion are sensed in the ATP hydrolysis domain.     

The specificity of the malarial VAR2CSA protein for chondroitin sulfate depends on 4-O-sulfation and ligand accessibility

Placental malaria infection is mediated by the binding of the malarial VAR2CSA protein to the placental glycosaminoglycan, chondroitin sulfate. Recombinant subfragments of VAR2CSA (rVAR2) have also been shown to bind specifically and with high affinity to cancer cells and tissues, suggesting the presence of a shared type of oncofetal chondroitin sulfate (ofCS) in the placenta and in tumors. However, the exact structure of ofCS and what determines the selective tropism of VAR2CSA remains poorly understood. In this study, ofCS was purified by affinity chromatography using rVAR2 and subjected to detailed structural analysis. We found high levels of N-acetylgalactosamine 4-O-sulfation (∼80–85%) in placenta- and tumor-derived ofCS. This level of 4-O-sulfation was also found in other tissues that do not support parasite sequestration, suggesting that VAR2CSA tropism is not exclusively determined by placenta- and tumor-specific sulfation. Here, we show that both placenta and tumors contain significantly more chondroitin sulfate moieties of higher molecular weight than other tissues. In line with this, CHPF and CHPF2, which encode proteins required for chondroitin polymerization, are significantly upregulated in most cancer types. CRISPR/Cas9 targeting of CHPF and CHPF2 in tumor cells reduced the average molecular weight of cell-surface chondroitin sulfate and resulted in a marked reduction of rVAR2 binding. Finally, utilizing a cell-based glycocalyx model, we showed that rVAR2 binding correlates with the length of the chondroitin sulfate chains in the cellular glycocalyx. These data demonstrate that the total amount and cellular accessibility of chondroitin sulfate chains impact rVAR2 binding and thus malaria infection.     

Relevance of forage fish in the diet of Magellanic penguins breeding in northern Patagonia,Argentina

We quantified the trophic niche of Magellanic penguins (Spheniscus magellanicus) breeding and moulting in Golfo San Jorge, Argentina, through conventional stomach content and stable isotope analysis. A total of 112 adults were flushed during the early and late chick stages of 2011 and 2012 at Isla Vernacci Norte, and at least 15 prey taxa were found, including fishes, cephalopods, crustaceans and polychaetes. Overall, Argentine anchovy (Engraulis anchoita) showed the highest contribution in terms of importance by mass (68.1–85.3%, depending on chick stage and year), except for the old chick stage in 2011 when the shortfin squid (Illex argentinus) was the main prey consumed (56.0%). Based on carbon and nitrogen isotopic values from a total of 256 blood samples, corresponding to young and old chicks and to adults of both sexes sampled throughout the incubation, chick and moult stages at the above mentioned colony and years, Bayesian mixing model outputs showed that Argentine anchovy was always the main prey (48–86%). Bayesian mixing model outputs obtained from adults of both sexes and their chicks during the late chick stage of 2013 at Isla Vernacci Norte, Isla Tova and Isla Leones also showed that Argentine anchovy was the main prey consumed. This is the first comprehensive assessment of Magellanic penguin diet composition in northern Patagonia, quantifying the relative contribution of prey in the diet of adults and chicks at different stages of the annual cycle and years, and confirms the relevance of a forage fish such as the Argentine anchovy in its trophic ecology.     

The Fragile X Mental Retardation Protein in Circadian Rhythmicity and Memory Consolidation

The control of new protein synthesis provides a means to locally regulate the availability of synaptic components necessary for dynamic neuronal processes. The fragile X mental retardation protein (FMRP), an RNA-binding translational regulator, is a key player mediating appropriate synaptic protein synthesis in response to neuronal activity levels. Loss of FMRP causes fragile X syndrome (FraX), the most commonly inherited form of mental retardation and autism spectrum disorders. FraX-associated translational dysregulation causes wide-ranging neurological deficits including severe impairments of biological rhythms, learning processes, and memory consolidation. Dysfunction in cytoskeletal regulation and synaptic scaffolding disrupts neuronal architecture and functional synaptic connectivity. The understanding of this devastating disease and the implementation of meaningful treatment strategies require a thorough exploration of the temporal and spatial requirements for FMRP in establishing and maintaining neural circuit function.     

Label-Free Protein Quantification for Plant Golgi Protein Localization and Abundance

The proteomic composition of the Arabidopsis (Arabidopsis thaliana) Golgi apparatus is currently reasonably well documented; however, little is known about the relative abundances between different proteins within this compartment. Accurate quantitative information of Golgi resident proteins is of great importance: it facilitates a better understanding of the biochemical processes that take place within this organelle, especially those of different polysaccharide synthesis pathways. Golgi resident proteins are challenging to quantify because the abundance of this organelle is relatively low within the cell. In this study, an organelle fractionation approach targeting the Golgi apparatus was combined with a label-free quantitative mass spectrometry (data-independent acquisition method using ion mobility separation known as LC-IMS-MS^E [or HDMS^E]) to simultaneously localize proteins to the Golgi apparatus and assess their relative quantity. In total, 102 Golgi-localized proteins were quantified. These data show that organelle fractionation in conjunction with label-free quantitative mass spectrometry is a powerful and relatively simple tool to access protein organelle localization and their relative abundances. The findings presented open a unique view on the organization of the plant Golgi apparatus, leading toward unique hypotheses centered on the biochemical processes of this organelle.The plant Golgi apparatus plays an important role in protein and lipid glycosylation and sorting as well as biosynthesis of large amounts of extracellular polysaccharides. It contains a large and diverse set of glycosyltransferases and other enzymes that are required for the synthesis and modification of these polysaccharides (Parsons et al., 2012b; Oikawa et al., 2013). The protein composition of this organelle has been the focus of a number of studies; however, these studies largely report a catalog of Golgi-localized proteins, and to date, there are no comprehensive data on the relative abundance of the different protein constituents of the Golgi apparatus (Dunkley et al., 2004, 2006; Sadowski et al., 2008; Nikolovski et al., 2012; Groen et al., 2014). The quantification of the plant Golgi proteome has been considered challenging, because this organelle is proportionally of low abundance in the cell; therefore, its constituent proteins are rarely identified in conventional proteomics experiments. Investigation of such low-abundance proteins generally requires sample fractionation on the organelle, protein, or peptide level (Stasyk and Huber, 2004; Haynes and Roberts, 2007; Di Palma et al., 2012).Here, an organelle fractionation approach in conjunction with label-free quantitative proteomic analysis was used to assess the localization and relative abundance of proteins within the plant Golgi apparatus. Label-free quantification is an increasingly popular alternative to isotopic tagging quantitative methods; it does not require labeling reagents and can be applied to an unlimited number of samples (Neilson et al., 2011; Evans et al., 2012). This is particularly appealing within plant proteomics, because the most conventional labeling strategy, Stable Isotope Labeling by Amino Acids in Cell Culture, is not easily suited for quantitative plant proteomic studies. The average labeling efficiency achieved using exogenous amino acid supply to Arabidopsis (Arabidopsis thaliana) cell cultures was found to be only 70% to 80% (Gruhler et al., 2005). Quantitative strategies with ¹⁵N metabolic labeling have been described for plant proteome analysis; however, care should be taken to ensure complete ¹⁵N incorporation, because even small amounts of ¹⁴N in the labeled sample can have significant detrimental effects on the number of peptide identifications (Nelson et al., 2007; Guo and Li, 2011; Arsova et al., 2012).In all label-free methods, samples under comparison are analyzed during separate mass spectrometry (MS) experiments (Neilson et al., 2011). The information from identified peptides is then used for relative and/or absolute quantification. The simplest label-free method involves taking the number of spectra acquired and assigned to peptides from the same protein as a measure of abundance (Ishihama et al., 2005). In an alternative approach, ion current recorded for a peptide ion is used as a measure of its abundance. The assumption is made that ion intensity is proportional to peptide amount in the sample analyzed, which holds true for nanoflow and microflow liquid chromatography (LC) systems (Levin et al., 2011; Christianson et al., 2013). Comparing peptide ion current between samples is, thus, widely used for relative quantification (Silva et al., 2005). To allow such comparison, a peptide must be identified across all samples under investigation, which is often challenging in LC-MS experiments given the highly complex nature of proteomics samples that contain tens of thousands of different peptides (Michalski et al., 2011). Hence, most relative ion intensity-based label-free approaches usually involve a step of identification transfer (Pasa-Tolíc et al., 2004). This involves matching ions from different acquisitions (in one of which, the ion has not been identified and is assigned the sequence from its matching pair in the other acquisition).Additionally, label-free proteomics can be used for absolute quantification (i.e. to estimate abundance of different proteins relative to each other within a given sample). Several different approaches have been suggested on how to convert peptide intensities to protein amounts (for comparison, see Wilhelm et al., 2014). One of the first such methods was Top-3 described by Silva et al. (2006b), who made a notable and unexpected observation, stating that the average MS signal response for the three most abundant peptides per 1 mol of protein is constant within a coefficient of variation of less than 10% (Silva et al., 2006b).In all these approaches, the peptide ion current is typically computed as the area under the curve of the chromatographic elution profile that is reconstituted from separate MS1 survey scans in which intact precursors are recorded. Determining a chromatographic profile accurately requires that the MS1 scans are performed at optimal frequency (Lange et al., 2008) and for optimal duration to record the MS1 signal at a high signal-to-noise ratio. In typical data-dependent acquisitions, however, the mass spectrometer oscillates between MS1 survey scans recording the mass/charge (m/z) for precursor peptide ions and then, a series of MS2 scans fragmenting one peptide ion precursor at a time, producing fragmentation spectra necessary for identification (Sadygov et al., 2004). As a result, the duration and frequency of MS2 scans determine the identification rate in data-dependent acquisition experiments but compromise time spent in MS1 required for accurate area under the curve quantification. Several groups have suggested data-independent acquisition, in which individual peptide ions are not selected for fragmentation but rather, groups of peptides of similar m/z are fragmented together. The exact number of cofragmented precursors depends on the speed and sensitivity of instrument configuration (for review, see Law and Lim, 2013). The simplest approach involves alternating between low-energy and high-energy scans of equal duration; low-energy scans record precursor peptide ions, whereas in high-energy scans, all precursors entering the mass spectrometer are cofragmented, and their fragments are recorded simultaneously. The method was called MS^E for Waters qTOF Mass Spectrometers (Geromanos et al., 2009) or all-ion fragmentation for Thermo Orbitrap Mass Spectrometers (Geiger et al., 2010). The analysis required downstream of this type of data acquisition is challenging given that the information of fragment origin (i.e. from what precursor peptide ion fragment was generated) is lost completely and that the high number of coeluting peptides is expected to create highly overlapping fragment spectra on fragmentation. To address this problem, Hoaglund-Hyzer and Clemmer (2001) have suggested fractionating peptides by ion mobility separation before fragmentation and MS and assigning fragments to precursors based on similarity of both chromatographic and mobility profiles (Hoaglund-Hyzer and Clemmer, 2001). The method was termed parallel fragmentation, and since that time, it has been commercialized by Waters as IMS-MS^E or HDMS^E (Shliaha et al., 2013).To date, the application of label-free quantitative proteomics to plant biology has been very limited. Recently, Helm et al. (2014) applied the LC-IMS-MS^E with Top-3 quantification to quantify the Arabidopsis chloroplast stroma proteome, allowing quantitative modeling of chloroplast metabolism. Two other works used the LC-MS^E method to assess the quantitative changes of cytosolic ribosomal proteins in response to Suc feeding and the extracellular proteome in response to salicylic acid (Cheng et al., 2009; Hummel et al., 2012).A number of proteomics approaches have been described to assess protein localization on a large scale (for review, see Gatto et al., 2010). Purification approaches attempt to isolate organelles to high levels of purity and subsequently identify and quantify proteins using LC-MS; however, such attempts yield limiting success and high false discovery rates (Andersen et al., 2002; Parsons et al., 2012a). A known limitation of this technique is the inability to completely isolate an organelle of interest, which combined with high proteome dynamic range, can result in some more abundant contaminants being identified and quantified at higher amounts than the target organelle residents. Moreover, even if a target organelle could be isolated to a certain degree of purity, it would still be impossible to deconvolute organelle residents from transient proteins that traffic through the target organelle. This becomes especially challenging for the organelles of the secretory pathway. To address these challenges, several groups applied fractionation of all organelles by gradient centrifugation and subsequent protein quantification by LC-MS. This produces distributions across the gradient for all quantified proteins, which are then used to assign organelle localization based on the specific distributions of organelle marker proteins. This effectively solves the problem of organelle contamination and protein trafficking, because a protein is expected to have a distribution characteristic of its organelle of residence, even if it is identified in all fractions, including those enriched in other organelles. Current variations of this method differ mostly by the LC-MS strategy used for quantification; for example, spectral counting was applied for protein-correlating profiles (Andersen et al., 2003), isobaric mass tagging (Nikolovski et al., 2012) and isotope-coded affinity tagging (Dunkley et al., 2004) were applied for localization of organelle proteins by isotope tagging (LOPIT), and Stable Isotope Labeling by Amino Acids in Cell Culture was applied for nucleolus/nucleus/cytosolic fractionation (Boisvert and Lamond, 2010).Here, a label-free LC-IMS-MS^E method was used for the analysis of density ultracentrifugation fractions enriched for the Golgi apparatus. First, we use relative label-free quantification involving identification transfer using the previously published synapter algorithm (Bond et al., 2013) to assess distributions of Golgi-localized proteins across the density gradient. These distributions are significantly different from those of residents of other organelles, which results in unambiguous protein assignment to the Golgi apparatus by multivariate data analysis. Second, the Top-3 absolute quantification method as implemented in Protein Lynx Global Server (PLGS) was used to rank order the Golgi-localized proteins by abundance in the fraction most enriched for Golgi apparatus. In conclusion, we present the analysis of protein distribution and abundances of the Golgi apparatus-enriched portion of the ultracentrifugation density gradient, allowing for simultaneous protein quantification and localization and leading to the assessment of relative abundances of 102 Golgi-localized proteins.     

Zinc to cadmium replacement in the A. thaliana SUPERMAN Cys₂ His₂ zinc finger induces structural rearrangements of typical DNA base determinant positions

Among heavy metals, whose toxicity cause a steadily increasing of environmental pollution, cadmium is of special concern due to its relatively high mobility in soils and potential toxicity at low concentrations. Given their ubiquitous role, zinc fingers domains have been proposed as mediators for the toxic and carcinogenic effects exerted by xenobiotic metals. To verify the structural effects of zinc replacement by cadmium in zinc fingers, we have determined the high resolution structure of the single Cys₂His₂ zinc finger of the Arabidopsis thaliana SUPERMAN protein (SUP37) complexed to the cadmium ion by means of UV–vis and NMR techniques. SUP37 is able to bind Cd(II), though with a dissociation constant higher than that measured for Zn(II). Cd‐SUP37 retains the ββα fold but experiences a global structural rearrangement affecting both the relative orientation of the secondary structure elements and the position of side chains involved in DNA recognition: among them Ser17 side chain, which we show to be essential for DNA binding, experiences the largest displacement. © 2011 Wiley Periodicals, Inc. Biopolymers 95: 801‐810, 2011.     

EBI2 operates independently of but in cooperation with CXCR5 and CCR7 to direct B cell migration and organization in follicles and the germinal center

Migration of B cells within lymphoid follicles is controlled by the chemokine receptors CXCR5 and CCR7 and the G-protein-coupled receptor EBI2 (GPR183). Whereas CXCR5 and CCR7 are known to mediate migration toward their respective chemokine ligands, it is unclear whether EBI2 acts by modulating these processes or by directly mediating chemotaxis toward its own spatially restricted ligand. It is also unknown how signals from these three receptors are integrated to control B cell localization. To answer these questions, we generated compound knockout mice deficient in expression of EBI2, CXCR5, or CCR7. Analysis of these mice revealed that EBI2 mediates B cell migration toward the outer areas of follicles and to bridging channels of the spleen independent of both CXCR5 and CCR7. Migratory signals delivered by EBI2 were shown to control B cell organization within the spleen and to be particularly important for positioning activated B cells in the early stages of Ab responses. An additional minor role for EBI2 was identified in the organization and affinity maturation of B cells in germinal centers. Thus, EBI2-mediated chemotaxis provides a third dimension to B cell migration that balances and integrates with the inputs from CXCR5 and CCR7 to determine B cell positioning.     

B-CePs as cross-linking probes for the investigation of RNA higher-order structure

Elucidating the structure of RNA and RNA ensembles is essential to understand biological functions. In this work, we explored the previously uncharted reactivity of bis-chloropiperidines (B-CePs) towards RNA. We characterized at the molecular level the different adducts induced by the fast reacting compound B-CeP 1 with RNA. Following an approach based on solution thermal melting coupled with ESI mass spectrometry (STHEM-ESI), we proved the ability of B-CePs to induce inter-molecular cross-links between guanines in double stranded RNA. These results open the possibility of using B-CePs as structural probes for investigating higher-order structures, such as the kissing loop complex established by the dimerization initiation site (DIS) of the HIV-1 genome. We confirmed the potential of B-CePs to reveal the identity of RNA structures involved in long-range interactions, expecting to benefit the characterization of samples that are not readily amenable to traditional high-resolution techniques, and thus promoting the elucidation of pertinent RNA systems associated with old and new diseases.