Genetic linkage map of the guppy,Poecilia reticulata,and quantitative trait loci analysis of male size and colour variation

We report construction of a genetic linkage map of the guppy genome using 790 single nucleotide polymorphism markers, integrated from six mapping crosses. The markers define 23 linkage groups (LGs), corresponding to the known haploid number of guppy chromosomes. The map, which spans a genetic length of 899 cM, includes 276 markers linked to expressed genes (expressed sequence tag), which have been used to derive broad syntenic relationships of guppy LGs with medaka chromosomes. This combined linkage map should facilitate the advancement of genetic studies for a wide variety of complex adaptive phenotypes relevant to natural and sexual selection in this species. We have used the linkage data to predict quantitative trait loci for a set of variable male traits including size and colour pattern. Contributing loci map to the sex LG for many of these traits.     

Formation of Self-organized Silver Nanocup-Type Structures and Their Plasmonic Absorption

The present work reports on the formation of extremely low volume, silver nanocup-type structures on the surface by annealing of ultra-thin silver film on quartz in inert environment. Atomic force microscopy studies together with scanning electron microscopy confirmed the formation of Ag nanocup-type structures at the surface. A basic physical model for the formation of nanocups in terms of buckling and Oswald ripening due to surface-induced morphological instability and diffusional mass transport under thermal treatment is demonstrated. Surface plasmon resonance absorptions of nanocup structures are studied and preliminary experiment for observing the surface-enhanced Raman scattering of fullerene C₇₀ molecules has been shown.     

Plasmodium falciparum UvrD Helicase Translocates in 3′ to 5′ Direction,Colocalizes with MLH and Modulates Its Activity through Physical Interaction

Malaria is a global disease and a major health problem. The control of malaria is a daunting task due to the increasing drug resistance. Therefore, there is an urgent need to identify and characterize novel parasite specific drug targets. In the present study we report the biochemical characterization of parasite specific UvrD helicase from Plasmodium falciparum. The N-terminal fragment (PfUDN) containing UvrD helicase domain, which consists of helicase motifs Q, Ia–Id, II, III and most of motif IV, and the C-terminal fragment (PfUDC1) containing UvrD helicase C terminal domain, consisting of remaining part of motif IV and motifs IVa–IVc and 161 amino acids of intervening sequence between motif IV and V, possess ssDNA-dependent ATPase and DNA helicase activities in vitro. Using immunodepletion assays we show that the ATPase and helicase activities are attributable to PfUDN and PfUDC1 proteins. The helicase activity can utilize the hydrolysis of all the nucleotide and deoxynucleotide triphosphates and the direction of unwinding is 3′ to 5′. The endogenous P. falciparum UvrD contains the characteristic DNA helicase activity. PfUDN interacts with PfMLH (P. falciparum MutL homologue) and modulates the endonuclease activity of PfMLH and PfMLH positively regulates the unwinding activity of PfUDN. We show that PfUvrD is expressed in the nucleus distinctly in the schizont stages of the intraerythrocytic development of the parasite and it colocalizes with PfMLH. These studies will make an important contribution in understanding the nucleic acid transaction in the malaria parasite.     

Plasmonic Tuning of Photoluminescence from Semiconducting Quantum Dot Assemblies

We report tuning of photoluminescence enhancement and quenching from closed packed monolayers of cadmium selenide quantum dots doped with gold nanoparticles. Plasmon-mediated control of the emission intensity from the monolayers is achieved by varying the size and packing density of the quantum dots as well as the doping concentration of gold nanoparticles. We observe a unique packing density dependent crossover from enhancement to quenching and vice versa for fixed size of quantum dots and doping concentration of gold nanoparticles. We suggest that this behavior is indicative of a crossover from single particle to collective emission from quantum dots mediated by gold nanoparticles.     

Homotopy semi-numerical simulation of peristaltic flow of generalised Oldroyd-B fluids with slip effects

This investigation deals with the peristaltic flow of generalised Oldroyd-B fluids (with the fractional model) through a cylindrical tube under the influence of wall slip conditions. The analysis is carried out under the assumptions of long wavelength and low Reynolds number. Analytical approximate solutions are obtained by using the highly versatile and rigorous semi-numerical procedure known as the homotopy analysis method. It is assumed that the cross section of the tube varies sinusoidally along the length of the tube. The effects of the dominant hydromechanical parameters, i.e. fractional parameters, material constants, slip parameter, time and amplitude on the pressure difference across one wavelength, are studied. Graphical plots reveal that the influence of both fractional parameters on pressure is opposite to each other. Interesting responses to a variation in the constants are obtained. Pressure is shown to be reduced by increasing the slip parameter. Furthermore, the pressure in the case of fractional models (fractional Oldroyd-B model and fractional Maxwell model) of viscoelastic fluids is considerably more substantial than that in the corresponding classical viscoelastic models (Oldroyd-B and Maxwell models). Applications of the study arise in biophysical food processing, embryology and gastro-fluid dynamics.     

Effect of forest fragment size on tree diversity and population structure of humid subtropical forest of Meghalaya,India

The present study was conducted in subtropical humid forests of Meghalaya to study the distributional pattern of species, floristic composition, community structure and tree population structure.Forest fragments of varying sizes(0.5 ha, 1 ha, 2 ha and 5 ha) were used in the study.All of the forest fragments are distributed within the same altitudinal range, and had similar rainfall and temperature regimes.Four forest fragments were sampled using random quadrats to analyze the impact of fragment size on tree...     

Methanogenic diversity studies within the rumen of Surti buffaloes based on methyl coenzyme M reductase A (mcrA) genes point to Methanobacteriales

Methane emissions from ruminant livestock are considered to be one of the more potent forms of greenhouse gases contributing to global warming. Many strategies to reduce emissions are targeting the methanogens that inhabit the rumen, but such an approach can only be successful if it targets all the major groups of ruminant methanogens. Therefore, basic knowledge of the diversity of these microbes in breeds of buffalo is required. Therefore, the methanogenic community in the rumen of Surti buffaloes was analyzed by PCR amplification, cloning, and sequencing of methyl coenzyme M reductase (mcrA) gene. A total of 76 clones were identified, revealing 14 different sequences (phylotypes). All 14 sequences were similar to methanogens belonging to the order Methanobacteriales. Within Methanobacteriales, 12 clones (6 OTUs) were similar to Methanosphaera stadtmanae and the remaining 8 phylotypes (64 clones) were similar to unclassified Methanobacteriales. Overall, members of the Methanobacteriales dominated the mcrA clone library in the rumen of Surti buffalo. Further studies and effective strategies can be made to inhibit the growth of Methanobacteriales to reduce methane emission from the rumen which would help in preventing global warming.     

Network based analysis of hepatitis C virus core and NS4B protein interactions

Hepatitis C virus (HCV) is a major cause of chronic liver disease worldwide. Here we attempt to further our understanding of the biological context of protein interactions in HCV pathogenesis, by investigating interactions between HCV proteins Core and NS4B and human host proteins. Using the yeast two-hybrid (Y2H) membrane protein system, eleven human host proteins interacting with Core and 45 interacting with NS4B were identified, most of which are novel. These interactions were used to infer overall protein interaction maps linking the viral proteins with components of the host cellular networks. Core and NS4B proteins contribute to highly compact interaction networks that may enable the virus to respond rapidly to host physiological responses to HCV infection. Analysis of the interaction networks highlighted enriched biological pathways likely influenced in HCV infection. Inspection of individual interactions offered further insights into the possible mechanisms that permit HCV to evade the host immune response and appropriate host metabolic machinery. Follow-up cellular assays with cell lines infected with HCV genotype 1b and 2a strains validated Core interacting proteins ENO1 and SLC25A5 and host protein PXN as novel regulators of HCV replication and viral production. ENO1 siRNA knockdown was found to inhibit HCV replication in both the HCV genotypes and viral RNA release in genotype 2a. PXN siRNA inhibition was observed to inhibit replication specifically in genotype 1b but not in genotype 2a, while SLC25A5 siRNA facilitated a minor increase in the viral RNA release in genotype 2a. Thus, our analysis can provide potential targets for more effective anti-HCV therapeutic intervention.