Effect of dietary selenium on the response of stressed and unstressed chickens toEscherichia coli challenge and antigen

Selenium was added to the feed of White Leghorn type chickens 1 day prior to challenge with eitherEscherichia coli or sheep erythrocyte antigen. the incidence of death or lesions was reduced from 86% to 21% at the optimal dose of selenium (0.4 mg/kg resulting in feed concentration of 0.45 mg/kg). After the chickens were stressed by chilling, selenium was ineffective againstE. coli. Dietary additions of selenium between 0.1 and 0.8 mg/kg resulted in an antibody titer increase from 2.2 to 3.9 to the log₂ against sheep erythrocytes (SRBC). Followng chilling, antibody titer response was reduced from 4.9 to 2.4 to the log₂. This titer reduction could be prevented with dietary additions of selenium between 0.1 and 1.2 mg/kg. The effects of a nitrofuran and selenium were additive againstE. coli challenge infection.     

Phototrophs in High-Iron-Concentration Microbial Mats: Physiological Ecology of Phototrophs in an Iron-Depositing Hot Spring

At Chocolate Pots Hot Springs in Yellowstone National Park the source waters have a pH near neutral, contain high concentrations of reduced iron, and lack sulfide. An iron formation that is associated with cyanobacterial mats is actively deposited. The uptake of [¹⁴C]bicarbonate was used to assess the impact of ferrous iron on photosynthesis in this environment. Photoautotrophy in some of the mats was stimulated by ferrous iron (1.0 mM). Microelectrodes were used to determine the impact of photosynthetic activity on the oxygen content and the pH in the mat and sediment microenvironments. Photosynthesis increased the oxygen concentration to 200% of air saturation levels in the top millimeter of the mats. The oxygen concentration decreased with depth and in the dark. Light-dependent increases in pH were observed. The penetration of light in the mats and in the sediments was determined. Visible radiation was rapidly attenuated in the top 2 mm of the iron-rich mats. Near-infrared radiation penetrated deeper. Iron was totally oxidized in the top few millimeters, but reduced iron was detected at greater depths. By increasing the pH and the oxygen concentration in the surface sediments, the cyanobacteria could potentially increase the rate of iron oxidation in situ. This high-iron-content hot spring provides a suitable model for studying the interactions of microbial photosynthesis and iron deposition and the role of photosynthesis in microbial iron cycling. This model may help clarify the potential role of photosynthesis in the deposition of Precambrian banded iron formations.     

Disease-associated change in an amphibian life-history trait

Oecologia - Emerging pathogens can drive evolutionary shifts in host life-history traits, yet this process remains poorly documented in vertebrate hosts. Amphibian chytridiomycosis, caused by...     

Copepod foraging and predation risk within the surface layer during night-time feeding forays

Vertical distribution data seem to indicate that certain speciesof diel vertical migrating copepods avoid the surface high chlorophyll(Chl) region within coastal and estuarine environments, evenduring the night. Copepods may avoid this layer to reduce predationmortality, avoid advective loss or to avoid consuming too muchtoxic algae. We hypothesize that copepods make several intermittentfeeding ‘forays’ into shallow surface layers duringthe night, returning to intermediate depths between forays.Using an individual-based model (IBM) of Calanus pacificus,we examined the implications of this behavior on feeding successand mortality risk, and tested whether a practical field-samplingscheme would be able to detect foray-like behavior. In somecases, mortality of the foray-foraging copepods was up to 50%less than that of randomly behaving controls, for a given amountof food ingested. The trapping scheme devised should be ableto detect the occurrence of foray behavior (FB) in the fieldand should show differences in the gut contents of copepodsentering and leaving the uppermost food-rich layer. The presenceor absence of foray-like behavior significantly altered therelative concentration of copepods within various surface strataand thus could influence the temporal availability of copepodsas prey for the larvae and juveniles of several important managedfish species. This paper is one of six on the subject of the role of zooplanktonpredator–prey interactions in structuring plankton communities.     

Isolation and characterization of microsatellite loci in the intertidal sponge Halichondria panicea

GA‐ and CA‐enriched genomic libraries were constructed for the intertidal sponge Halichondria panicea. Unique repeat motifs identified varied from the expected simple dinucleotide repeats to more complex repeat units. All sequences tended to be highly repetitive but did not necessarily contain the targeted motifs. Seven microsatellite loci were evaluated on sponges from the clone source population. All seven were polymorphic with 5.43 ± 0.92 mean number of alleles. Six of the seven loci that could be resolved had mean heterozygosities of 0.14–0.68. The loci identified here will be useful for population studies.     

Toward visualization of nanomachines in their native cellular environment

The cellular nanocosm is made up of numerous types of macromolecular complexes or biological nanomachines. These form functional modules that are organized into complex subcellular networks. Information on the ultra-structure of these nanomachines has mainly been obtained by analyzing isolated structures, using imaging techniques such as X-ray crystallography, NMR, or single particle electron microscopy (EM). Yet there is a strong need to image biological complexes in a native state and within a cellular environment, in order to gain a better understanding of their functions. Emerging methods in EM are now making this goal reachable. Cryo-electron tomography bypasses the need for conventional fixatives, dehydration and stains, so that a close-to-native environment is retained. As this technique is approaching macromolecular resolution, it is possible to create maps of individual macromolecular complexes. X-ray and NMR data can be ‘docked’ or fitted into the lower resolution particle density maps to create a macromolecular atlas of the cell under normal and pathological conditions. The majority of cells, however, are too thick to be imaged in an intact state and therefore methods such as ‘high pressure freezing’ with ‘freeze-substitution followed by room temperature plastic sectioning’ or ‘cryo-sectioning of unperturbed vitreous fully hydrated samples’ have been introduced for electron tomography. Here, we review methodological considerations for visualizing nanomachines in a close-to-physiological, cellular context. EM is in a renaissance, and further innovations and training in this field should be fully supported. Robert Feulgen Lecture 2009 presented at the 51st symposium of the Society for Histochemistry in Stubai, Austria, October 7–10, 2009.     

Protonation of Individual Histidine Residues Is Not Required for the pH-Dependent Entry of West Nile Virus: Evaluation of the “Histidine Switch” Hypothesis

Histidine residues have been hypothesized to function as sensors of environmental pH that can trigger the activity of viral fusion proteins. We investigated a requirement for histidine residues in the envelope (E) protein of West Nile virus during pH-dependent entry into cells. Each histidine was individually replaced with a nonionizable amino acid and tested functionally. In each instance, mutants capable of orchestrating pH-dependent infection were identified. These results do not support a requirement for any single histidine as a pH-sensing “switch,” and they suggest that additional features of the E protein are involved in triggering pH-dependent steps in the flavivirus life cycle.Flaviviruses are enveloped RNA viruses that cause a spectrum of illnesses in humans ranging from fever to encephalitis and hemorrhagic disease (20). These small (∼50 nM) spherical virions incorporate 180 envelope (E) proteins that orchestrate the process of virus entry (22). Flaviviruses bind cells via poorly characterized receptors, are internalized by clathrin-mediated endocytosis (10), and fuse with the membranes of endosomal compartments in a pH-dependent fashion (18, 33). Upon exposure to mildly acidic conditions (∼pH 6.5), E proteins undergo extensive changes in conformation and oligomeric state that serve to tether viral and cellular membranes and pull them into the close apposition required to promote lipid mixing (12, 29). While this transformation has been detailed using biochemical and structural approaches (14, 22, 29), how an acidic environment triggers these events is less clear. The “histidine switch” hypothesis identifies a critical role for histidine residues as sensors that trigger the activity of viral fusion proteins that direct pH-dependent entry into cells (16, 21). The rationale for this theory is that histidine is unique among amino acids in that it becomes protonated and charged upon exposure to acidic environments similar to those that support viral fusion (the pK_a of histidine in proteins is ∼6.4) (32). Evidence in support of a required role for histidine residues in the conformational changes of viral proteins that direct membrane fusion has been obtained using several groups of viruses that enter cells in a pH-dependent fashion (4, 5, 9, 15, 27, 31).West Nile virus (WNV) is a mosquito-borne encephalitic flavivirus that has emerged during the last decade as a threat to public health in the Western hemisphere (3). To investigate a requirement for the ionization of histidine residues during WNV entry, we constructed a panel of mutants with histidine substitutions in the E protein and evaluated their capacity to mediate infection. The E protein is composed of three distinct domains (DI to DIII) that are connected to the viral membrane by a helical region called the stem-anchor (17, 24). Each of these protein regions contains histidine residues that could be involved in triggering conformational changes that drive pH-dependent membrane fusion (Fig. ​(Fig.1A).1A). Five of the 13 histidine residues in the E protein are completely conserved among flaviviruses. Each individual histidine was mutated to two different amino acids using QuikChange mutagenesis (Stratagene, La Jolla, CA). Alanine and glutamine substitutions were selected because the side chains of these amino acids are nonionizable (Fig. 1B to D).Open in a separate windowFIG. 1.Impact of mutations at individual histidine residues in the WNV E protein on virus infectivity. (A) The WNV E protein is composed of three structurally distinct domains (DI-DIII). There are 13 histidine residues in the E protein; 3 of these are located in DI (red ribbons), 4 in DII (yellow ribbons), 4 in DIII (blue ribbons), and 2 in the stem-anchor region that anchors the E protein to the viral membrane (not pictured). Five of these histidine residues are conserved among flaviviruses (labeled in red). (B to D) RVPs composed of E proteins incorporating alanine (red) or glutamine (green) histidine substitutions were produced by genetic complementation. The infectious titer of each preparation was determined following infection of Raji-DC-SIGNR cells with serial twofold dilutions of RVPs. Infection was scored as a function of reporter gene expression 48 h postinfection and was measured using flow cytometry. (E) The infectious titer of each glutamine substitution mutant in Raji-DC-SIGNR cells was calculated for multiple independent RVP preparations using data from linear portions of the virus dose/infectivity curves. Hatched bars show results for mutants with substitutions at conserved histidine residues. The means of the results for four or five independent RVP preparations are shown; error bars identify the standard errors. (F) The titers of glutamine substitution mutants were determined following infection of Vero cells with serial twofold dilutions of RVPs. The infectious titer of each mutant was calculated as described above. Hatched bars show results for mutants with substitutions at conserved histidine residues. The means of titers from four independent experiments are shown; error bars represent the standard errors.WNV reporter virus particles (RVPs) that incorporate each E protein mutant were produced by complementation as described previously (25, 26). Briefly, BHK-21 cells that propagate a subgenomic WNV replicon encoding green fluorescent protein were transfected with plasmids encoding WNV capsid and precursor to membrane (prM)-E proteins, followed by incubation for 2 days at 37°C. The titers of RVP preparations in Raji cells expressing the attachment factor DC-SIGNR were determined following infection with six serial twofold dilutions of virions (7). Because RVPs are capable of only a single round of infection and do not encapsidate a genome that encodes the E protein, there is no opportunity for reversion to the wild-type (WT) sequence during production. Analysis of the panel of mutants revealed three patterns (Fig. 1B to D and data not shown). Near-WT levels of infectivity were observed for mutants with both substitutions at four different histidine residues (H81, H320, H395, and H398) (Fig. ​(Fig.1B).1B). Analysis of multiple independent RVP preparations with glutamine substitutions indicated that, on average, the titer of RVPs incorporating these mutants was reduced by only ∼25% (n = 4 or 5 preparations) in comparison to the titer in preparations with WT E protein (Fig. ​(Fig.1E).1E). In contrast, neither substitution at position H144 or H246 yielded infectious virus particles (Fig. 1D and E). A third group of mutants displayed an intermediate phenotype with the degree of attenuation dependent upon the amino acid substitution (Fig. 1C and E). A similar pattern was observed when Vero cells were used to determine RVP titers (Fig. ​(Fig.1F).1F). While in several instances (H144 and H246) a glutamine substitution resulted in a significant reduction in the number of virus particles released from transfected cells, quantitative analysis of the E protein content of RVP preparations indicated that a simple failure to release virus particles is not sufficient to explain the reduction in infectious titer observed with each mutant (data not shown). A limitation of any mutagenesis approach is that negative results must be interpreted with caution. While the identification of functional substitutions that encode nonionizable amino acids rules out a requirement for histidine protonation at a given position during virus entry, mutations may also subtly affect E protein structure or functions not relating to sensing changes in endosomal pH.We next expanded our efforts to identify functional substitutions at positions H144 and H246. Additional mutants were constructed by site-directed mutagenesis employing primers encoding a random sequence (NNN) at the codons of H144 or H246. Because mutations may affect virus infectivity by modulating the efficiency of virion maturation, RVPs were produced in cells cotransfected with a plasmid expressing human furin, a condition shown previously to dramatically enhance the efficiency of prM cleavage (7, 23). Augmented furin expression in RVP-producing cells resulted in complete maturation of each mutant tested (data not shown), suggesting that the low-pH-mediated conformational changes that regulate exposure of the furin cleavage site are not dependent upon a single histidine residue. RVPs were also produced at both 37°C and 28°C; experiments at the latter temperature were performed to minimize the potential impact of mutations on E protein folding and stability. For substitutions at most histidine residues, overexpression of furin in producer cells had only a modest effect on the release of infectious RVPs relative to the level in control experiments with WT E proteins (data not shown; n = 3 or 4 preparations). Notably, conditions that promoted more efficient maturation resulted in a significant increase in the production of infectious RVPs incorporating the H144Q substitution (25-fold, P < 0.05), albeit at very low titers (Fig. ​(Fig.2A2A and data not shown; ∼1.4 × 10³ infectious units/ml at 37°C, n = 9). Analysis of seven additional H144 mutants identified asparagine (Fig. 2A and B) and methionine (data not shown) substitutions that could be incorporated into infectious virions. RVPs composed of the H144N mutant were produced at ∼1.4% and 31% (37°C and 28°C, respectively; n = 4) of the level observed in paired experiments with WT RVPs, and the levels were not significantly different in the presence or absence of furin overexpression despite relatively inefficient cleavage of prM of H144N in the absence of furin expression (data not shown). All 19 amino acid substitutions at H246 were analyzed, and substitutions with aromatic side chains (tryptophan, phenylalanine, and tyrosine) were identified as capable of orchestrating virus entry (Fig. 2C and D and data not shown). When produced at 28°C, the titer of H246F RVPs was reduced only ∼twofold relative to the titers in studies with WT RVPs. In agreement with these findings, a neutralization escape mutant of WNV encoding an H246Y mutation has recently been described (35). Altogether, these studies identified individual substitutions with nonionizable side chains at each of the 13 E protein histidine residues that can be incorporated into RVPs with significant infectious titers.Open in a separate windowFIG. 2.Identification of functional substitutions for H144 and H246. WNV RVPs incorporating E protein histidine substitution mutants were produced by complementation in the presence or absence of a plasmid expressing human furin, followed by incubation at 37°C (A and C) or 28°C (B and D) (1, 7, 23). The infectious titers of RVP populations were determined as described in the Fig. ​Fig.11 legend. All titer experiments were performed at 37°C, even when lower temperatures were used to produce the RVPs. The titers of RVPs produced in the presence of exogenous furin expression are shown by hatched bars. The means of the results of three or four independent experiments are displayed; error bars identify the standard errors. (E and F) Entry of WNV RVPs incorporating histidine mutants is pH dependent. Raji-DC-SIGNR cells were treated with serial dilutions of the weak base NH₄Cl (from 0.2 to 50 mM) for 5 to 10 min at room temperature prior to infection with RVPs. Cells were washed at 12 h postinfection and cultured for an additional 36 h in fresh medium. Infectivity was measured by flow cytometry at 48 h postinfection. The concentration of NH₄Cl required to inhibit infection by 50% (IC₅₀) was calculated by nonlinear regression. (F) The means of two or three independent measurements are shown; error bars represent the standard errors. Hatched bars show results for mutants with substitutions at conserved histidine residues.To confirm that virions composed of each functional mutant entered cells in a pH-dependent fashion, we next established that infectious entry could be inhibited by neutralization of endosomal compartments. Ammonium chloride is a lysosomotropic agent shown to block membrane fusion by pH-dependent viruses, including flaviviruses (10, 11, 13, 28, 34). Infection by each mutant was completely inhibited by NH₄Cl; the concentrations required to inhibit 50% of infection were calculated by nonlinear regression and found to be similar for WT WNV and histidine mutants (Fig. 2E and F).While our data suggest that no single histidine residue is required for E protein-mediated entry of WNV, it is possible that several act in concert. For example, ionization of multiple histidine residues is thought to trigger pH-dependent conformational changes in the fusion proteins of vesicular stomatitis virus and baculovirus (4, 15). The antiparallel arrangement of E proteins on the virion clusters H144, H152, and H320 at the hinge between DI and DII along the dimer interface of the E protein. Previous structural studies speculated that ionization of these three residues may trigger dimer disassociation following exposure to an acidic environment (2, 9, 24). Therefore, we constructed double and triple mutants containing substitutions in histidine residues at the DI-DII hinge and were able to identify combinations of mutations that allow for the production of infectious RVPs with significant titers (Fig. ​(Fig.3).3). While these data indicate that this cluster of histidine residues hypothesized previously to function as a pH sensor are not required for infection, it is certainly possible that other combinations of histidine (and nonhistidine) residues may coordinate to function in this regard.Open in a separate windowFIG. 3.Production of infectious RVPs incorporating multiple histidine substitutions at the DI-DII hinge. RVPs incorporating substitutions at one or more histidine positions clustered around the DI-DII hinge were produced by genetic complementation. The infectious titers of multiple independent preparations of RVPs were calculated as described in the Fig. ​Fig.11 legend. The means of two or three independent measurements are shown; error bars represent the standard errors.Recent studies of tick-borne encephalitis virus (TBEV) identified the conserved histidine at position 323 (corresponding to H320 of WNV) as the critical pH sensor required for the initiation of viral membrane fusion (9). Using a recombinant subviral particle (SVP) system (6, 8, 30), Fritz and colleagues found that TBEV SVPs incorporating a H323A mutation form unstable E protein trimers and are unable to fuse with synthetic liposomes when exposed to low pH (9). SVPs are small (∼30 nM), noninfectious virus-like particles composed of 60 E proteins that have been used extensively as a model of flavivirus fusion (29). Because our studies with WNV RVPs and a replication-competent infectious clone (data not shown) indicate that this residue is dispensable for pH-dependent infection, we explored this discrepancy by introducing mutations into the E protein of Langat virus (LGTV), a flavivirus that shares roughly 80% amino acid identity with TBEV. A panel of H146 and H323 mutants were produced using degenerate primers as described above and incorporated into RVPs composed of the replicon RNA and capsid protein of WNV. LGTV RVPs composed of H323L and H146R mutants were produced with titers similar to or greater than the titer of those incorporating WT LGTV E proteins (1.1 and 4.6 times the WT titer, respectively) (Fig. ​(Fig.4A).4A). In each case, RVP infection remained pH dependent (Fig. ​(Fig.4B).4B). How to reconcile the differences between our findings with WNV and LGTV and those reported for TBEV is unclear. One possibility is that the sensor of acidic pH differs between SVPs and infectious virions, perhaps due to differences in the geometry of these two classes of virus particles (T = 1 and pseudo-T = 3, respectively) (8, 19). Alternatively, the lipid-mixing assay used in vitro may be differentially sensitive to factors that affect the requirements for and efficiency of viral membrane fusion.Open in a separate windowFIG. 4.Mutation of conserved histidine residues in the tick-borne flavivirus LGTV. (A) A panel of mutants at positions H146 and H323 in LGTV was produced by QuikChange mutagenesis employing redundant primers. Mutants were assayed for their capacity to direct virus entry of RVPs produced by complementation. Multiple substitutions for positions H146 and H323 were capable of mediating entry of RVPs (data not shown). The titers of RVPs composed of H146R and H323L were calculated as described in the Fig. ​Fig.11 legend. The mean titers from three independent RVP preparations are shown; error bars represent the standard errors. (B) The pH dependence of LGTV RVP entry was confirmed as described in the Fig. ​Fig.22 legend. The means of two or three independent measurements are shown; error bars represent the standard errors.Histidine residues acquire a positive charge when exposed to the mildly acidic conditions known to trigger the fusion machinery of flaviviruses. In principle, these residues are uniquely suited to serve as sensors of environmental pH. However, our results indicate that there is no requirement for protonation of a particular “histidine switch” during the infectious entry of WNV, as mutagenesis studies identified viable substitutions with nonionizable side chains at all 13 histidine residues within the E protein. While not all the mutants identified were as infectious as WT RVPs, this is not particularly surprising, as any change away from the naturally selected WT sequence has the potential to affect protein structure or function. How the E protein senses a low-pH environment remains unclear and appears to require the contribution of additional amino acids. Because amino acid side-chain pK_a is influenced locally by protein structure, it is possible that nonhistidine residues are coordinated such that they are ionized at ∼pH 6.5. Resolving this complexity awaits further study.