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681 research outputs found

Mutations and SNPs of human cardiac sodium channel alpha subunit gene (SCN5A) in Japanese patients with Brugada syndrome

Author: Ackerman MJ Splawski I, Makielski
Aydin A Bahring S, Dahm S, Guenthe
Bezzina C Veldkamp MW, van Den Ber
Brugada P and Brugada J
Chen JZ Xie XD, Wang XX, Tao M, Sh
Furuhashi M Uno K, Tsuchihashi K,
Huang H Zhao J, Barrane FZ, Champa
Splawski I Shen J, Timothy KW, Leh
Wattanasirichaigoon D Vesely MR, D
Publication venue: 'Okayama Medical Association'
Publication date: 01/01/2007
Field of study

Background: Brugada syndrome is an inherited arrhythmogenic disease characterized by right bundle branch block pattern and ST segment elevation, leading to the change of V1 to V3 on electrocardiogram, and an increased risk of sudden cardiac death resulting from ventricular fibrillation. The sodium channel alpha 5 subunit (SCN5A) gene encodes a cardiac voltage-dependent sodium channel, and SCN5A mutations have been reported in Brugada syndrome. However, single nucleotide polymorphisms (SNPs) and gene mutations have not been well investigated in Japanese patients with Brugada syndrome. Methods and Results: The SCN5A gene was examined in 58 patients by using PCR and the ABI 3130xl sequencer, revealing 17 SNP patterns and 13 mutations. Of the 13 mutations, 8 were missense mutations (with amino acid change), 4 were silent mutations (without amino acid change), and one case was a mutation within the splicing junction. Six of the eight missense mutations were novel mutations. Interestingly, we detected an R1664H mutation, which was identified originally in long QT syndrome. Conclusion: We found 13 mutations of the SCN5A gene in 58 patients with Brugada syndrome. The disease may be attributable to some of the mutations and SNPs

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Okayama University Scientific Achievement Repository

Smc5/6 coordinates formation and resolution of joint molecules with chromosome morphology to ensure meiotic divisions

Author: A Chavez
A De Muyt
A Hochwagen
A Hochwagen
A Irmisch
A McAleenan
A Schwacha
A Sourirajan
A Svetlanov
AC Chan
AJ Wood
AL Marston
Alex D. Herbert
Alice Copsey
Andreas Hochwagen
Andrew Chi-ho Chan
B Rockmill
BH Lee
C Buhler
C Tapia-Alveal
DM Sheedy
E Ampatzidou
EA Andrews
EA Outwin
ER Hoffmann
Eva Hoffmann
F Osman
FZ Watts
G De Piccoli
G Vader
GA Cromie
GR Smith
GV Borner
H Murakami
Hannah G. Blitzblau
HB Lindroos
HG Blitzblau
HG Blitzblau
HG Yu
HG Yu
I Lilienthal
J Gregan
J Matos
J Matos
J Palecek
J Pan
J Torres-Rosell
J Zalevsky
JA Carballo
JA Downs
JK Holloway
JM Murray
JR Mullen
JR Mullen
JS Bickel
K Nishimura
K Zakharyevich
K Zakharyevich
KA Henderson
KP Kim
KP Kohl
KT Nishant
L Jessop
L Jessop
L Newnham
L Wu
L Xu
LE Berchowitz
LE Hang
LJ Gaskell
Louise Newnham
M Bermudez-Lopez
M Xaver
MA Roy
Michael Lichten
MJ Neale
MN Boddy
MS McMahill
N Hunter
N Hunter
N Wu
Neil Hunter
NK Kolas
O Yildiz
P Jordan
Philip W. Jordan
PR Potts
PR Potts
Prakash Arumugam
RK Clyne
S Agarwal
S Chu
S Farmer
S Gray
S Panizza
S Pebernard
S Wehrkamp-Richter
SB Buonomo
SD Oh
SD Oh
Shangming Tang
SL Andersen
Sonya Newcombe
Stephen Gray
T de los Santos
T Snowden
T Wechsler
TM Carlile
TS Kitajima
V Kaliraman
WM Fricke
X Zhao
Y Blat
YH Chen
YH Chen
Zhaobo Li
Publication venue: 'Public Library of Science (PLoS)'
Publication date: 01/01/2013
Field of study

During meiosis, Structural Maintenance of Chromosome (SMC) complexes underpin two fundamental features of meiosis: homologous recombination and chromosome segregation. While meiotic functions of the cohesin and condensin complexes have been delineated, the role of the third SMC complex, Smc5/6, remains enigmatic. Here we identify specific, essential meiotic functions for the Smc5/6 complex in homologous recombination and the regulation of cohesin. We show that Smc5/6 is enriched at centromeres and cohesin-association sites where it regulates sister-chromatid cohesion and the timely removal of cohesin from chromosomal arms, respectively. Smc5/6 also localizes to recombination hotspots, where it promotes normal formation and resolution of a subset of joint-molecule intermediates. In this regard, Smc5/6 functions independently of the major crossover pathway defined by the MutLγ complex. Furthermore, we show that Smc5/6 is required for stable chromosomal localization of the XPF-family endonuclease, Mus81-Mms4Eme1. Our data suggest that the Smc5/6 complex is required for specific recombination and chromosomal processes throughout meiosis and that in its absence, attempts at cell division with unresolved joint molecules and residual cohesin lead to severe recombination-induced meiotic catastroph

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The Francis Crick Institute

Subcellular fractionation method to study endosomal trafficking of KaposiÃ¢â‚¬â„¢s sarcoma-associated herpesvirus

Author: A Greiner
A Vonderheit
AL Feire
AS Hahn
B Chandran
B Hernaez
C Bandyopadhyay
CA Harley
FG Giancotti
FZ Wang
G Rappocciolo
GY Yu
H Zhao
HA Hussein
HH Krishnan
HJ Garrigues
J Grove
JY Yang
K Eto
KL Schornberg
L Hertel
LA Huber
LR Walker
M Barczyk
M Wolf
MG Waugh
MV Veettil
OF Dyson
PA Grange
Q Tang
S Bhattacharyya
S Chakraborty
SM Akula
SM Akula
SM Akula
SM Akula
SM Akula
T Braulke
T Iwahara
U Repnik
W Zhang
Y Yamauchi
Publication venue: 'Springer Science and Business Media LLC'
Publication date: 01/01/2016
Field of study

Background Virus entry involves multiple steps and is a highly orchestrated process on which successful infection collectively depends. Entry processes are commonly analyzed by monitoring internalized virus particles via Western blotting, polymerase chain reaction, and imaging techniques that allow scientist to track the intracellular location of the pathogen. Such studies have provided abundant direct evidence on how viruses interact with receptor molecules on the cell surface, induce cell signaling at the point of initial contact with the cell to facilitate internalization, and exploit existing endocytic mechanisms of the cell for their ultimate infectious agenda. However, there is dearth of knowledge in regards to trafficking of a virus via endosomes. Herein, we describe an optimized laboratory procedure to isolate individual organelles during different stages of endocytosis by performing subcellular fractionation. This methodology is established using Kaposiâ€™s sarcoma-associated herpesvirus (KSHV) infection of human foreskin fibroblast (HFF) cells as a model. With KSHV and other herpesviruses alike, envelope glycoproteins have been widely reported to physically engage target cell surface receptors, such as integrins, in interactions leading to entry and subsequent infection. Results Subcellular fractionation was used to isolate early and late endosomes (EEs and LEs) by performing a series of centrifugations steps. Specifically, a centrifugation step post-homogenization was utilized to obtain the post-nuclear supernatant containing intact intracellular organelles in suspension. Successive fractionation via sucrose density gradient centrifugation was performed to isolate specific organelles including EEs and LEs. Intracellular KSHV trafficking was directly traced in the isolated endosomal fractions. Additionally, the subcellular fractionation approach demonstrates a key role for integrins in the endosomal trafficking of KSHV. The results obtained from fractionation studies corroborated those obtained by traditional imaging studies. Conclusions This study is the first of its kind to employ a sucrose flotation gradient assay to map intracellular KSHV trafficking in HFF cells. We are confident that such an approach will serve as a powerful tool to directly study intracellular trafficking of a virus, signaling events occurring on endosomal membranes, and dynamics of molecular events within endosomes that are crucial for uncoating and virus escape into the cytosol

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