Higher plants use LOV to perceive blue light

Higher plants use several classes of blue light receptors to modulate a wide variety of physiological responses. Among them, both the phototropins and members of the Zeitlupe (ZTL) family use light oxygen voltage (LOV) photosensory domains. In Arabidopsis, these families comprise phot1, phot2 and ZTL, LOV Kelch Protein 2 (LKP2), and Flavin-binding Kelch F-box1 (FKF1). It has now been convincingly shown that blue-light-induced autophosphorylation of the phot1 kinase domain is an essential step in signal transduction. Recent experiments also shed light on the partially distinct photosensory specificities of phot1 and phot2. Phototropin signaling branches rapidly following photoreceptor activation to mediate distinct responses such as chloroplast movements or phototropism. Light activation of the LOV domain in ZTL family members modulates their capacity to interact with GIGANTEA (GI) and their ubiquitin E3 ligase activity. A complex between GI and FKF1 is required to trigger the degradation of a repressor of CO (CONSTANS) expression and thus modulates flowering time. In contrast, light-regulated complex formation between ZTL and GI appears to limit the capacity of ZTL to degrade its targets, which are part of the circadian oscillator.     

TIMP-1 binding to proMMP-9/CD44 complex localized at the cell surface promotes erythroid cell survival

Besides its ability to inhibit MMP activity, TIMP-1 exhibits other biological functions. We earlier reported that TIMP-1 induced UT-7 erythroid cell survival through activation of the JAK2/PI 3-kinase/Akt pathway and we now aim to determine whether the TIMP-1 anti-apoptotic effect requires MMP involvement. We first show that proMMP-9 was expressed in UT-7 cells and associated with the cell plasma membrane. Such proMMP-9 localization was crucial for TIMP-1 intracellular signalling since (i) TIMP-1 specifically bound to proMMP-9 and (ii) proMMP-9 silencing abrogated the TIMP-1 effect. We also demonstrated that TIMP-1 anti-apoptotic effect was independent on MMP inhibition since MMP-9 function blocking antibodies as well as a synthetic MMP inhibitor were unable to reproduce TIMP-1 effect. Nevertheless, these compounds prevented TIMP-1 binding to proMMP-9 and subsequently abolished TIMP-1-induced cell survival. We finally demonstrated that CD44 anchored proMMP-9 to the plasma membrane and enabled TIMP-1-mediated signal transduction. Therefore, our results indicate that the anti-apoptotic signalling of TIMP-1 depends on the formation of a ternary complex between TIMP-1, proMMP-9 and CD44 at the UT-7 erythroid cell surface.     

The town Crepis and the country Crepis: How does fragmentation affect a plant–pollinator interaction?

In fragmented habitats, one cause of the decrease of plant diversity and abundance is the disruption of plant–animal interactions, and in particular plant–pollinator interactions. Since habitat fragmentation acts both on pollinator behaviour and plant reproduction, its consequences for the stability of such interactions are complex. An extreme case of habitat fragmentation occurs in urbanised areas where suitable habitat (in the present study small patches around ornamental trees) is embedded in a highly unsuitable environment (concrete matrix). Based on simple experiments, we ask whether pollinators can adapt their foraging behaviour in response to the amount of available resources (flowers) in the fragments and their isolation, as predicted by the optimal foraging theory. To do so we analysed the effect of fragmentation on the behaviour of pollinators visiting Crepis sancta (L.) Bornm. (Asteraceae), which forms large populations in the countryside and patchy populations in urban environments. More precisely we studied pollinator visitation rates, capitulum visit durations, capitulum search durations and capitulum size choice. Pollinators chose larger capitula in both types of populations and their foraging behaviour differed between the two population types in three ways: (1) pollinator visits were lower in urban fragmented populations, perhaps due to the lower accessibility of urban patches; (2) capitulum visit durations were longer in urban fragmented populations, a possible compensation of energy lost during flights among patches; and (3) capitulum search durations where longer in urban fragmented populations, which may represent an increase in capitulum prospecting effort. We discuss the possible impacts of such differences for plant population functioning in the two types of populations.     

Synthesis of phosphatidylcholine, a typical eukaryotic phospholipid, is necessary for full virulence of the intracellular bacterial parasite Brucella abortus

Phosphatidylcholine (PC) is a typical eukaryotic phospholipid absent from most prokaryotes. Thus, its presence in some intracellular bacteria is intriguing as it may constitute host mimicry. The role of PC in Brucella abortus was examined by generating mutants in pcs (BApcs) and pmtA (BApmtA), which encode key enzymes of the two bacterial PC biosynthetic routes, the choline and methyl-transferase pathways. In rich medium, BApcs and the double mutant BApcspmtA but not BApmtA displayed reduced growth, increased phosphatidylethanolamine and no PC, showing that Pcs is essential for PC synthesis under these conditions. In minimal medium, the parental strain, BApcs and BApmtA showed reduced but significant amounts of PC suggesting that PmtA may also be functional. Probing with phage Tb, antibiotics, polycations and serum demonstrated that all mutants had altered envelopes. In macrophages, BApcs and BApcspmtA showed reduced ability to evade fusion with lysosomes and establish a replication niche. In mice, BApcs showed attenuation only at early times after infection, BApmtA at later stages and BApcspmtA throughout. The results suggest that Pcs and PmtA have complementary roles in vivo related to nutrient availability and that PC and the membrane properties that depend on this typical eukaryotic phospholipid are essential for Brucella virulence.     

Synthesis of multiarm star poly(glycerol)-block-poly(2-hydroxyethyl methacrylate)

Well-defined multiarm star block copolymers poly(glycerol)-b-poly(2-hydroxyethyl methacrylate) (PG-b-PHEMA) with an average of 56, 66, and 90 PHEMA arms, respectively, have been prepared by atom transfer radical polymerization (ATRP) of HEMA in methanol by a core-first strategy. The hyperbranched macroinitiators employed were prepared on the basis of well-defined hyperbranched polyglycerol by esterification with 2-bromoisobutyryl bromide. Polydispersites M(w)/M(n) of the new multiarm stars were in the range of 1.11-1.82. Unexpectedly, with the combination of CuCl/CuBr(2)/2,2'-bipyridyl as catalyst, the polymerization conversion can be driven to maximum values of 79%. The control of CuCl catalyst concentration is also very important to achieve high conversion and narrow polydispersity. The absolute M(n) values of the obtained multiarm star polymers were in good agreement with the calculated ones, and the highest M(n) values of the multiarm star copolymer is around 10(6) g/mol. Kinetic analysis shows that an induction period exists in the polymerization of HEMA. After this induction period, a linear dependence of ln ([M](0)/[M](t)()) on time was observed. Due to the star architecture, the viscosity of the obtained multiarm star PHEMA is much lower than that of linear PHEMA.     

Limited Interference at the Early Stage of Infection between Two Recombinant Novirhabdoviruses: Viral Hemorrhagic Septicemia Virus and Infectious Hematopoietic Necrosis Virus

The genome sequence of a hypervirulent novirhabdovirus, viral hemorrhagic septicemia virus (VHSV) French strain 23-75, was determined. Compared to the genome of the prototype Fil3 strain, a number of substitutions, deletions, and insertions were observed. Following the establishment of a plasmid-based minigenome replication assay, recombinant VHSV (rVHSV) was successfully recovered. rVHSV exhibits wild-type-like growth properties in vitro as well as in vivo in rainbow trout. The dispensable role of NV for the novirhabdovirus replication was confirmed by generating rVHSV-ΔNV, in which the NV gene was deleted. This deletion mutant was shown to be as debilitated as that previously described for infectious hematopoietic necrosis virus (IHNV), a distantly related novirhabdovirus (S. Biacchesi, M. I. Thoulouze, M. Bearzotti, Y. X. Yu, and M. Bremont, J. Virol. 74:11247-11253, 2000). Recombinant VHSV and IHNV expressing tdTomato and GFP_max reporter genes, respectively, were generated, demonstrating the potential of these rhabdoviruses to serve as viral vectors. Interestingly, rIHNV-GFP_max could be recovered using the replicative complex proteins of either virus, whereas rVHSV-Tomato could be recovered only by using its own replicative complex, reflecting that the genome signal sequences of VHSV are relatively distant from those of IHNV and do not allow their cross-recognition. Moreover, the use of heterologous protein combinations underlined the importance of strong protein-protein interactions for the formation of a functional ribonucleoprotein complex. The rIHNV-GFP_max and rVHSV-Tomato viruses were used to simultaneously coinfect cell monolayers. It was observed that up to 74% of the cell monolayer was coinfected by both viruses, demonstrating that a limited interference phenomenon exists during the early stage of primary infection, and it was not mediated by a cellular antiviral protein or by some of the viral proteins.Viral hemorrhagic septicemia virus (VHSV) is a member of the Novirhabdovirus genus in the Rhabdoviridae family. VHSV is considered by many countries and international organizations to be one of the most important viral pathogens of finfish (38). During recent years, VHSV has been isolated from at least 50 different species from marine and freshwater fish and is present throughout the northern hemisphere (45). The transmission of the virus from fish to fish occurs directly through the water or by contact between infected and healthy individuals. VHSV is thought to enter the body through the gills or possibly through wounds on the skin. However, we recently showed that fins may represent the main portal of entry for the novirhabdoviruses (25). The virus usually causes severe hemorrhages in the skin, muscles, eyes, kidney, and liver, with mortality rates as high as 90%. As for all members of the Rhabdoviridae family, the VHSV genome consists of a negative-sense single-stranded RNA molecule of about 11 kb encoding five structural proteins: N, the nucleoprotein; P, a polymerase-associated protein; M, the matrix protein; G, the unique viral surface glycoprotein; and L, the large RNA-dependent RNA polymerase. In addition, like the other members of the Novirhabdovirus genus, such as infectious hematopoietic necrosis virus (IHNV), the VHSV genome encodes a small nonstructural NV protein, which has been shown to be dispensable for IHNV replication in cell culture and is involved in virus-induced pathogenicity in rainbow trout (8, 50).The sequence analysis of the glycoprotein (G) and nucleoprotein (N) genes of VHSV has shown that VHSV isolates can be divided into four genotypes that generally correlate with geographic location rather than the host species (4, 19, 47, 49). Isolates belonging to VHSV genotypes I, II, and III are present in continental Europe, the north Atlantic Ocean, the Baltic Sea, the North Sea, and waters around Scotland. Genotype IV consists of isolates from the marine environment in North America. Recently, viral hemorrhagic septicemia has become an emerging disease of freshwater fish in the Great Lakes region of North America (2, 54). Thus, it is quite obvious that VHSV is becoming a worldwide and very-broad-host-range fish virus and that the development of efficient vaccines is needed. Reverse genetics, allowing the introduction of targeted modifications into the viral genome and the production of attenuated live vaccine, may help to fight this rapidly spreading and emerging virus. It is routinely observed in farm trouts exposed to viral diseases that VHSV and IHNV coexist (26). By developing experimental coinfections by VHSV and IHNV in rainbow trout, Brudeseth et al. studied the pathogenesis and virus distribution (10). They found that both viruses established an infection and raised similar virus titers in kidneys, but the distribution of IHNV was more restricted in internal organs during the acute stage of the infection and was not detected in the brain. However, it generally is admitted that infection by one virus renders host cells resistant to a superinfecting virus.Superinfection exclusion, also known as homologous interference, is the phenomenon in which a cell infected with one type of virus or transfected with a viral replicon becomes resistant to a secondary infection with the same virus, whereas infection with unrelated viruses normally is unaffected (40, 51). Superinfection exclusion has been observed in a broad range of viruses, including vaccinia virus (14, 18), human immunodeficiency virus (HIV) (36, 37), vesicular stomatitis virus (VSV) (32, 43, 53), Borna disease virus (BDV) (24), measles virus (34), Sindbis virus (28), Semliki Forest virus (44), rubella virus (15), hepatitis C virus (HCV) (40, 51), and bovine viral diarrhea virus (BVDV) (31). Mechanisms of exclusion are diverse and have not been determined in all cases, but mechanisms described so far are caused by competition among different viruses for critical replicative pathways (for example, the use of the same receptors for the entry) or depend on the direct interaction of products of the primary infection with the secondary infecting virus. For example, the superinfection exclusion of VSV was found to be caused by a combination of three distinct effects on endocytosis by VSV-infected cells: (i) a decreased rate of the formation of endocytic vesicles, (ii) a decreased rate of the internalization of receptor-bound ligands, and (iii) a competition with newly synthesized virus for the occupancy of coated pits (43). In contrast, the cytoplasmic accumulation of BDV nucleocapsid components appeared to prevent subsequent infection through a blockage of the polymerase activity of incoming viruses (24). Superinfection exclusion by BVDV was the result of dual mechanisms that were mediated by the structural protein E2, which blocks the entry of a homologous second virus, and by a blockage at the level of replication dependent on the level of primary viral RNA replication but not influenced by the expression of viral structural proteins, as observed for BDV (31). HIV employs its early gene product Nef to efficiently interfere with superinfection at the virus entry step by downregulating cell surface receptors (36). Finally, vaccinia virus expresses in newly infected cells two surface proteins that mark cells as infected and induce the repulsion of superinfecting viruses (18).In the present study, we described a reverse-genetics system for VHSV allowing the generation of a wild-type-like recombinant VHSV and a recombinant virus expressing a red fluorescent protein (Tomato). The system is based on the French strain 23/75 of VHSV, which is a hypervirulent and devastating strain for farmed rainbow trout belonging to genotype I (serotype III) and was isolated in France in 1975 from a brown trout (16, 23). Thus, this system provides a suitable starting point for identifying potential virulence determinants, as demonstrated by the deletion of the NV gene, and for developing attenuated derivatives as candidate vaccines. Using the available reverse-genetics system elaborated with IHNV, a recombinant IHNV expressing a green fluorescent protein (GFP) also was produced (8), and it was of interest to study whether a superinfection exclusion phenomenon could be observed between both VHSV and IHNV, whose cohabitation has been recorded often. We showed that up to 74% of a cell monolayer could be simultaneously infected by the viruses, demonstrating a limited viral interference between salmonid novirhabdoviruses and that, based on previous data, chimeric or pseudotyped viruses could be generated (6).