Optimization of Path Selection in MIMO

Multi-hop communication is the best way for improving the coverage area with reduced transmission power.This paper can easily found a path selection based on multi-hop decode and forward (DF) cooperative system. Then it is said to be a simple parallel multi-hop paths based cooperative communication system. Recently, cooperative communication have attracted significant attention to tackle the limitations imposed by multiple-input-multiple-output (MIMO) technology. To eliminate these limitations and increase spectral efficiency, Compress-and-Forward(CF) technique was proposed. In many known examples where compress-and-forward(CF) for relay networks is capacity achieving, it is only trivially so, i.e., it falls back to hashing without quantization.A potentially better strategy is to decode as much as possible and to compress the residual information, i.e., a combination of decode-and-forward (DF) and CF

PERFORMANCE ANALYSIS OF AN ENERGY EFFICIENT FFT PROCESSOR USING 32nm CMOS TECHNOLOGY

ABSTRACT This paper presents an energy-efficient Fast Fourier Transform (FFT) processor which meets the requirements of DSP applications. Fast Fourier Transform is one of the widely used digital signals processing (DSP) algorithms which analysis the signal in its frequency domain. Modified DOMS-FF (Duration Observation Master Slave-Flip Flop) is introduced to reduce the power dissipation and makes the computation of the result much faster than the existing system. The goal of this work is to get less area and energy efficient FFT processor with build in all requirements necessary for DSP applications

αA-crystallin R49Cneo mutation influences the architecture of lens fiber cell membranes and causes posterior and nuclear cataracts in mice

<p>Abstract</p> <p>Background</p> <p>αA-crystallin (CRYAA/HSPB4), a major component of all vertebrate eye lenses, is a small heat shock protein responsible for maintaining lens transparency. The R49C mutation in the αA-crystallin protein is linked with non-syndromic, hereditary human cataracts in a four-generation Caucasian family.</p> <p>Methods</p> <p>This study describes a mouse cataract model generated by insertion of a neomycin-resistant (neo^r) gene into an intron of the gene encoding mutant R49C αA-crystallin. Mice carrying the neo^rgene and wild-type <it>Cryaa </it>were also generated as controls. Heterozygous knock-in mice containing one wild type gene and one mutated gene for αA-crystallin (WT/R49C^neo) and homozygous knock-in mice containing two mutated genes (R49C^neo/R49C^neo) were compared.</p> <p>Results</p> <p>By 3 weeks, WT/R49C^neomice exhibited large vacuoles in the cortical region 100 μm from the lens surface, and by 3 months posterior and nuclear cataracts had developed. WT/R49C^neomice demonstrated severe posterior cataracts at 9 months of age, with considerable posterior nuclear migration evident in histological sections. R49C^neo/R49C^neomice demonstrated nearly complete lens opacities by 5 months of age. In contrast, R49C mice in which the neo^rgene was deleted by breeding with CreEIIa mice developed lens abnormalities at birth, suggesting that the neo^rgene may suppress expression of mutant R49C αA-crystallin protein.</p> <p>Conclusion</p> <p>It is apparent that modification of membrane and cell-cell interactions occurs in the presence of the αA-crystallin mutation and rapidly leads to lens cell pathology <it>in vivo</it>.</p

Mutations within the cGMP-binding domain of CNGA1 causing autosomal recessive retinitis pigmentosa in human and animal model.

Retinitis pigmentosa is a group of progressive inherited retinal dystrophies that may present clinically as part of a syndromic entity or as an isolated (nonsyndromic) manifestation. In an Indian family suffering from retinitis pigmentosa, we identified a missense variation in CNGA1 affecting the cyclic nucleotide binding domain (CNBD) and characterized a mouse model developed with mutated CNBD. A gene panel analysis comprising 105 known RP genes was used to analyze a family with autosomal-recessive retinitis pigmentosa (arRP) and revealed that CNGA1 was affected. From sperm samples of ENU mutagenesis derived F1 mice, we re-derived a mutant with a Cnga1 mutation. Homozygous mutant mice, developing retinal degeneration, were examined for morphological and functional consequences of the mutation. In the family, we identified a rare CNGA1 variant (NM_001379270.1) c.1525 G &gt; A; (p.Gly509Arg), which co-segregated among the affected family members. Homozygous Cnga1 mice harboring a (ENSMUST00000087213.12) c.1526 A &gt; G (p.Tyr509Cys) mutation showed progressive degeneration in the retinal photoreceptors from 8 weeks on. This study supports a role for CNGA1 as a disease gene for arRP and provides new insights on the pathobiology of cGMP-binding domain mutations in CNGA1-RP