A biomolecule friendly photolithographic process for fabrication of protein microarrays on polymeric films coated on silicon chips

The last years, there is a steadily growing demand for methods and materials appropriate to create patterns of biomolecules for bioanalytical applications. Here, a photolithographic method for patterning biomolecules onto a silicon surface coated with a polymeric layer of high protein binding capacity is presented. The patterning process does not affect the polymeric film and the activity of the immobilized onto the surface biomolecules. Therefore, it permits sequential immobilization of different biomolecules on spatially distinct areas on the same solid support. The polymeric layer is based on a commercially available photoresist (AZ5214) that is cured at high temperature in order to provide a stable substrate for creation of protein microarrays by the developed photolithographic process. The photolithographic material consists of a (meth)acrylate copolymer and a sulfonium salt as a photoacid generator, and it is lithographically processed by thermal treatment at temperatures 相似文献   

Inhibition of Anopheles gambiae Odorant Receptor Function by Mosquito Repellents

The identification of molecular targets of insect repellents has been a challenging task, with their effects on odorant receptors (ORs) remaining a debatable issue. Here, we describe a study on the effects of selected mosquito repellents, including the widely used repellent N,N-diethyl-meta-toluamide (DEET), on the function of specific ORs of the African malaria vector Anopheles gambiae. This study, which has been based on quantitative measurements of a Ca²⁺-activated photoprotein biosensor of recombinant OR function in an insect cell-based expression platform and a sequential compound addition protocol, revealed that heteromeric OR (ORx/Orco) function was susceptible to strong inhibition by all tested mosquito repellents except DEET. Moreover, our results demonstrated that the observed inhibition was due to efficient blocking of Orco (olfactory receptor coreceptor) function. This mechanism of repellent action, which is reported for the first time, is distinct from the mode of action of other characterized insect repellents including DEET.     

Fungal Endopolygalacturonases Are Recognized as Microbe-Associated Molecular Patterns by the Arabidopsis Receptor-Like Protein RESPONSIVENESS TO BOTRYTIS POLYGALACTURONASES1

Plants perceive microbial invaders using pattern recognition receptors that recognize microbe-associated molecular patterns. In this study, we identified RESPONSIVENESS TO BOTRYTIS POLYGALACTURONASES1 (RBPG1), an Arabidopsis (Arabidopsis thaliana) leucine-rich repeat receptor-like protein, AtRLP42, that recognizes fungal endopolygalacturonases (PGs) and acts as a novel microbe-associated molecular pattern receptor. RBPG1 recognizes several PGs from the plant pathogen Botrytis cinerea as well as one from the saprotroph Aspergillus niger. Infiltration of B. cinerea PGs into Arabidopsis accession Columbia induced a necrotic response, whereas accession Brno (Br-0) showed no symptoms. A map-based cloning strategy, combined with comparative and functional genomics, led to the identification of the Columbia RBPG1 gene and showed that this gene is essential for the responsiveness of Arabidopsis to the PGs. Transformation of RBPG1 into accession Br-0 resulted in a gain of PG responsiveness. Transgenic Br-0 plants expressing RBPG1 were equally susceptible as the recipient Br-0 to the necrotroph B. cinerea and to the biotroph Hyaloperonospora arabidopsidis. Pretreating leaves of the transgenic plants with a PG resulted in increased resistance to H. arabidopsidis. Coimmunoprecipitation experiments demonstrated that RBPG1 and PG form a complex in Nicotiana benthamiana, which also involves the Arabidopsis leucine-rich repeat receptor-like protein SOBIR1 (for SUPPRESSOR OF BIR1). sobir1 mutant plants did not induce necrosis in response to PGs and were compromised in PG-induced resistance to H. arabidopsidis.Microbe-associated molecular patterns (MAMPs) are molecular signatures of entire groups of microbes and have key roles in activation of the defense response in plants (Jones and Dangl, 2006; Boller and Felix, 2009). Well-characterized proteinaceous MAMPs are bacterial flagellin, Elongation Factor Tu (EF-Tu), and Ax21, fungal xylanase, and oomycete pep13, an epitope of a secreted transglutaminase (Boller and Felix, 2009; Monaghan and Zipfel, 2012). Plants recognize MAMPs by means of pattern recognition receptors (PRRs), comprising a group of leucine-rich repeat (LRR) receptor-like kinases (RLKs) or LRR receptor-like proteins (RLPs) located in the plasma membrane (Greeff et al., 2012; Monaghan and Zipfel, 2012). The LRR-RLKs FLS2 and EFR recognize flg22 (the 22-amino acid eliciting epitope from the conserved flagellin domain) and elf18/elf26 (peptides derived from the N terminus of translation elongation factor EF-Tu), respectively (Gómez-Gómez and Boller, 2000; Kunze et al., 2004; Chinchilla et al., 2006; Zipfel et al., 2006). The fungal protein ethylene-inducing xylanase (EIX) is recognized by the tomato (Solanum lycopersicum) LRR-RLPs LeEIX1 and LeEIX2, of which only the latter mediates a necrotic response (Ron and Avni, 2004).BRI1-ASSOCIATED KINASE1/SOMATIC EMBRYOGENESIS RECEPTOR KINASE3 (BAK1/SERK3) is an LRR-RLK acting as a common component in many RLK signaling complexes (Monaghan and Zipfel, 2012). Although it was originally identified as a protein that interacts with the brassinosteroid receptor BRI1 (Li et al., 2002; Nam and Li, 2002), BAK1 also forms ligand-induced complexes with FLS2 and EFR and contributes to disease resistance against the pathogens Pseudomonas syringae, Hyaloperonospora arabidopsidis (Hpa), and Phytophthora infestans (Chinchilla et al., 2007; Heese et al., 2007; Chaparro-Garcia et al., 2011; Roux et al., 2011). Tomato BAK1 interacts in a ligand-independent manner with LeEIX1 but not with LeEIX2, and the BAK1-LeEIX1 interaction is required for the ability of LeEIX1 to attenuate the signaling of LeEIX2 (Bar et al., 2010). BAK1 has also been shown to interact with another LRR-RLK, BAK1-INTERACTING RECEPTOR-LIKE KINASE1 (BIR1). A bir1 mutant showed extensive cell death, activation of constitutive defense responses, and impairment in the activation of the mitogen-activated protein kinase MPK4 (Gao et al., 2009). sobir1 (for suppressor of BIR1) mutants suppress BIR1 phenotypes, and overexpression of SOBIR1 triggers cell death and defense responses (Gao et al., 2009). SOBIR1 does not physically interact with BIR1, suggesting that SOBIR1 mediates an alternative signal transduction route. A recent study showed that the tomato SOBIR1 interacts with RLPs and is required for RLP-mediated disease resistance (Liebrand et al., 2013).Endopolygalacturonases (PGs) are a class of pectinases that hydrolyze the homogalacturonan domain of pectic polysaccharides (van den Brink and de Vries, 2011). Secreted PGs are able to cause cell wall decomposition and tissue maceration and thereby act as virulence factors in several fungal pathogens, such as Aspergillus flavus, Claviceps purpurea, and Alternaria citri (Shieh et al., 1997; Isshiki et al., 2001; Oeser et al., 2002). The most extensively studied PGs from fungal plant pathogens are those of Botrytis cinerea (for review, see Zhang and van Kan, 2013b), a necrotrophic broad-host-range pathogen that contains six PG genes (designated Bcpg1–Bcpg6) in its genome (Wubben et al., 1999). Deletion of either Bcpg1 or Bcpg2 resulted in a strong reduction in virulence on tomato and broad bean (Vicia faba) leaves (ten Have et al., 1998; Kars et al., 2005), presumably because the enzymes have a detrimental effect on the integrity of host cell walls and tissues. Indeed, infiltrating BcPG2 into broad bean leaves or transient expression of BcPG2 in Nicotiana benthamiana led to tissue collapse and necrosis, and the necrotic response was abolished when the catalytic domain of the PG was mutated (Kars et al., 2005; Joubert et al., 2007). By contrast, Poinssot et al. (2003) reported that BcPG1 can activate plant defense responses in grapevine (Vitis vinifera) cell suspensions independently of its enzymatic activity, suggesting that the protein itself might be recognized by plant cells as an elicitor. These studies with seemingly opposing conclusions were conducted with different isozymes on distinct cell types of different plant species. Thus, it remained inconclusive whether plant responses observed after exposure to PGs are due to the structural damage resulting from pectin hydrolysis or to recognition of the protein as a MAMP (followed by downstream signaling responses).The degradation of pectin by PGs leads to the release of oligogalacturonides (OGAs), which may activate a variety of defense responses (Prade et al., 1999; D’Ovidio et al., 2004). OGAs act as damage-associated molecular patterns (DAMPs) via their perception by the cell wall-associated receptor Wall-Associated Kinase1 (WAK1; Brutus et al., 2010). Overexpression of WAK1 in Arabidopsis (Arabidopsis thaliana) enhances resistance to B. cinerea (Brutus et al., 2010).Here, we describe the occurrence of natural variation among Arabidopsis accessions in responsiveness to fungal PGs. Two accessions that strongly differed in their response to PGs were selected for further analysis. Cloning and functional characterization demonstrated that the gene RESPONSIVENESS TO BOTRYTIS POLYGALACTURONASES1 (RBPG1) encodes an LRR-RLP. Finally, we demonstrate that the LRR-RLK SUPPRESSOR OF BIR1 (SOBIR1) interacts with RBPG1 and is essential for responsiveness to fungal PGs.     

Development and homeostasis of the skin epidermis

The skin epidermis is a stratified epithelium that forms a barrier that protects animals from dehydration, mechanical stress, and infections. The epidermis encompasses different appendages, such as the hair follicle (HF), the sebaceous gland (SG), the sweat gland, and the touch dome, that are essential for thermoregulation, sensing the environment, and influencing social behavior. The epidermis undergoes a constant turnover and distinct stem cells (SCs) are responsible for the homeostasis of the different epidermal compartments. Deregulation of the signaling pathways controlling the balance between renewal and differentiation often leads to cancer formation.     

Identification of hake distribution pattern and nursery grounds in the Hellenic seas by means of generalized additive models

A time series of hake abundance data obtained from the “MEDITS” experimental surveys carried out in the Greek seas from 1996 to 2006 have been modeled by means of Generalized Additive Models (GAMs), as functions of spatial and temporal variables, including sampling position (latitude–longitude interaction), depth, and year. All variables were highly significant but most of the variation was explained by the sampling position and the depth. Total abundance was higher in the 100–450 m depth zone, while juveniles showed preference for shallower waters, being more abundant from 100 to 320 m. Model predictions were used to generate density distributions maps, which revealed that total abundance is relatively higher in the western part of the Aegean Sea and in the eastern part of the Cretan Sea, while its maximum values are expected in the Saronikos Gulf. Nursery grounds are restricted in specific regions with the most important of them being in the Saronikos Gulf and its surrounding area. Guest editor: V. D. Valavanis Essential Fish Habitat Mapping in the Mediterranean     

Intra-species variation in transient accumulation of leaf anthocyanins in Cistus creticus during winter: evidence that anthocyanins may compensate for an inherent photosynthetic and photoprotective inferiority of the red-leaf phenotype

Leaf color in some individuals of Cistus creticus turns transiently to red during winter, while neighboring individuals occupying the same site remain green. We have examined whether anthocyanin accumulation can be associated with variations in photosynthetic and/or photoprotective characteristics between the two phenotypes, rendering the red phenotype more vulnerable to photoinhibition and, accordingly, needing additional protection in the form of anthocyanins. Towards this aim, maximum (pre-dawn) and effective (mid-day) PSII photochemical efficiencies, xanthophyll cycle pool sizes and leaf nitrogen contents were seasonably followed, encompassing both the green (spring, summer, autumn) and the red (winter) period of the year. Moreover, the distribution of the two phenotypes in exposed and shaded sites was assessed. The frequency of red individuals was considerably higher in fully exposed sites, pointing to a photoprotective function of leaf anthocyanins. Yet, the assumption was not corroborated by pre-dawn PSII yield measurements, since both phenotypes displayed similar high values throughout the year and a similar drop during winter. However, the red phenotype was characterized by lower light-saturated PSII yields, xanthophyll cycle pool sizes and leaf nitrogen, during both the green and the red period of the year. Based on this correlative evidence, we suggest that winter redness in C. creticus may compensate for an inherent photosynthetic and photoprotective inferiority, possibly through a light screen and/or an antioxidant function of leaf anthocyanins.     

Thrombin mediates mitogenesis and survival of human endothelial cells through distinct mechanisms

Thrombin has been reported to play a pivotal role in the initiation of angiogenesis by indirectly regulating and organizing a network of angiogenic molecules. In addition, it has been proposed that thrombin can directly activate endothelial cell proliferation. However, in this report it was shown that thrombin is a poor growth factor for human endothelial cells, and its modest mitogenic activity is mediated indirectly by the release of heparin-binding epidermal growth factor, subsequent to proteinase-activated receptor 1 (PAR1) activation. On the other hand, it was demonstrated that thrombin is a potent anti-apoptotic factor for endothelial cells, pointing to a novel role of thrombin in vascular protection. Analysis by annexin V-propidium iodide double staining revealed that thrombin, specifically, promoted survival of serum-starved endothelial cells in a concentration-dependent manner. In contrast to its mitogenic effect, the anti-apoptotic effect of thrombin was largely independent of its catalytic activity and was mediated through interaction with alphanubeta3 and alpha5beta1 integrins, whereas the involvement of PAR1 was limited. These results provide new insights in understanding the role of thrombin in endothelial cell signaling and vascular biology.     

Red leaf color as a warning signal against insect herbivory: Honest or mimetic?

The co-evolution theory for red leaf colors considers redness as a handicap signal against herbivory. We have examined whether the assumed signal is honest and, accordingly, costly, by seeking a correlation between anthocyanin and total phenolic levels in 11 plants exhibiting variation in the expression of the red character either between individuals or between modules on the same individual. Selection of total phenolics as a variable was based on their assumed anti-herbivore function and on their common biosynthetic origin with anthocyanins. Plants with young or senescing red leaves were tested. Confirming evidence was found in senescing leaves, where in three out of the four studied species a significant and strongly positive correlation between signal strength (redness) and actual defensive potential (total phenolics) was found, rendering the signal both honest and costly. In young, developing leaves a significant, yet weakly positive correlation was found only in three out the seven examined species. Accordingly, the handicap signal hypothesis may be questioned in the case of young leaves. Hence, young leaf redness fits more to the alternative hypotheses that red leaf color is less easily perceived by folivorous insect photoreceptors or that red leaf color undermines insect camouflage. These hypotheses do not demand an increased chemical defensive potential.     

Sad3 and sad4 are required for saponin biosynthesis and root development in oat

Avenacins are antimicrobial triterpene glycosides that are produced by oat (Avena) roots. These compounds confer broad-spectrum resistance to soil pathogens. Avenacin A-1, the major avenacin produced by oats, is strongly UV fluorescent and accumulates in root epidermal cells. We previously defined nine loci required for avenacin synthesis, eight of which are clustered. Mutants affected at seven of these (including Saponin-deficient1 [Sad1], the gene for the first committed enzyme in the pathway) have normal root morphology but reduced root fluorescence. In this study, we focus on mutations at the other two loci, Sad3 (also within the gene cluster) and Sad4 (unlinked), which result in stunted root growth, membrane trafficking defects in the root epidermis, and root hair deficiency. While sad3 and sad4 mutants both accumulate the same intermediate, monodeglucosyl avenacin A-1, the effect on avenacin A-1 glucosylation in sad4 mutants is only partial. sad1/sad1 sad3/sad3 and sad1/sad1 sad4/sad4 double mutants have normal root morphology, implying that the accumulation of incompletely glucosylated avenacin A-1 disrupts membrane trafficking and causes degeneration of the epidermis, with consequential effects on root hair formation. Various lines of evidence indicate that these effects are dosage-dependent. The significance of these data for the evolution and maintenance of the avenacin gene cluster is discussed.     

Validated method for the simultaneous determination of methadone and its main metabolites (EDDP and EMDP) in plasma of umbilical cord blood by gas chromatography-mass spectrometry

A sensitive and specific GC/MS method for the determination of methadone (MDN) and its two main metabolites, 2-ethylidene-1,5-dimethyl-3,3-diphenylpyrrolidine (EDDP) and 2-ethyl-5-methyl-3,3-diphenylpyrroline (EMDP), in plasma samples obtained from venous and arterial umbilical cord blood and maternal blood has been developed, optimized and validated. Specimen preparation includes protein precipitation with acetonitrile and simultaneous solid-phase extraction of the three analytes. Methadone-d9 was used as internal standard for the determination of MDN and EMDP, while EDDP-d3 for EDDP. Limits of detection were 0.6 microg/L for MDN and 0.3 microg/L for EDDP and EMDP, while limits of quantification were 2.0 microg/L for MDN and 1.0 microg/L for EDDP and EMDP. The calibration curves were linear up to 2000 microg/L for MDN and up to 1000 microg/L for EDDP and EMDP. Absolute recovery ranged from 94.8 to 99.7% for all three analytes. Intra- and interday accuracy was less than 5.3 and 5.5%, respectively, while intra- and interday precision was less than 3.5 and 5.0%, correspondingly, for all analytes. The method proved suitable for the determination of MDN and its two main metabolites in plasma samples obtained from umbilical cord and maternal blood of a woman participating in a MDN maintenance program, during the prenatal and postpartum period.