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Structural, Functional, and Spectroscopic Characterization of the Substrate Scope of the Novel Nitrating Cytochrome P450 TxtE

Author: Arnold Frances H.
Brinkmann-Chen Sabine
Cahn Jackson K. B.
Dodani Sheel C.
Heinisch Tillmann
McIntosh John A.
Publication venue: 'Royal College of Obstetricians & Gynaecologists (RCOG)'
Publication date: 13/10/2014
Field of study

A novel cytochrome P450 enzyme, TxtE, was recently shown to catalyze the direct aromatic nitration of L-tryptophan. This unique chemistry inspired us to ask whether TxtE could serve as a platform for engineering new nitration biocatalysts to replace current harsh synthetic methods. As a first step toward this goal, and to better understand the wild-type enzyme, we obtained high-resolution structures of TxtE in its substrate-free and substrate-bound forms. We also screened a library of substrate analogues for spectroscopic indicators of binding and for production of nitrated products. From these results, we found that the wild-type enzyme accepts moderate decoration of the indole ring, but the amino acid moiety is crucial for binding and correct positioning of the substrate and therefore less amenable to modification. A nitrogen atom is essential for catalysis, and a carbonyl must be present to recruit the αB′1 helix of the protein to seal the binding pocket

The genetic interaction network of CCW12, a Saccharomyces cerevisiae gene required for cell wall integrity during budding and formation of mating projections

Author: A Boorsma
A Herscovics
A Lagorce
A Lagorce
AH Tong
AH Tong
AI Saeed
B Santos
C Bermejo
C Cappellaro
C Carotti
C Huttenhower
CB Brachmann
CE Bulawa
Christine Neupert
CJ Roberts
D Sheikh-Hamad
DE Levin
DJ DeMarini
E Cabib
E Cabib
E Ragni
Enrico Ragni
F Hutzler
FM Klis
G Lesage
G Lesage
GJ Smits
GJ Smits
H Iida
H Kojima
Heidi Piberger
HL Piao
I Gagnon-Arsenault
I Hagen
J Burke
J Chant
J Sambrook
J Trueheart
JA Hadwiger
JA Trilla
JA Trilla
Javier Arroyo
Jesús García-Cantalejo
JJ Heinisch
JL Brown
JS Robinson
K Madden
KK Lam
Laura Popolo
LJ Oehlen
M Costanzo
M Ecker
M Rajavel
M Rep
M Schmidt
M Watanabe
MA Leza
Markus Aebi
MH Valdivieso
O Protchenko
PA Delley
PW De Groot
PW De Groot
QY Yin
R García
R García
R Green
R Kollár
R Schmitt
RA Arkowitz
RJ Rothstein
S Shankarnarayan
Sabine Strahl
T Zu
TH Nguyen
TR Hughes
US Jung
V Mrsa
V Wood
WR Parrish
XL Zhan
Publication venue: BioMed Central
Publication date: 01/01/2011
Field of study

Abstract Background Mannoproteins construct the outer cover of the fungal cell wall. The covalently linked cell wall protein Ccw12p is an abundant mannoprotein. It is considered as crucial structural cell wall component since in baker's yeast the lack of <it>CCW12 </it>results in severe cell wall damage and reduced mating efficiency. Results In order to explore the function of <it>CCW12</it>, we performed a Synthetic Genetic Analysis (SGA) and identified genes that are essential in the absence of <it>CCW12</it>. The resulting interaction network identified 21 genes involved in cell wall integrity, chitin synthesis, cell polarity, vesicular transport and endocytosis. Among those are <it>PFD1</it>, <it>WHI3</it>, <it>SRN2</it>, <it>PAC10</it>, <it>FEN1 </it>and <it>YDR417C</it>, which have not been related to cell wall integrity before. We correlated our results with genetic interaction networks of genes involved in glucan and chitin synthesis. A core of genes essential to maintain cell integrity in response to cell wall stress was identified. In addition, we performed a large-scale transcriptional analysis and compared the transcriptional changes observed in mutant <it>ccw12</it>Δ with transcriptomes from studies investigating responses to constitutive or acute cell wall damage. We identified a set of genes that are highly induced in the majority of the mutants/conditions and are directly related to the cell wall integrity pathway and cell wall compensatory responses. Among those are <it>BCK1</it>, <it>CHS3</it>, <it>EDE1</it>, <it>PFD1</it>, <it>SLT2 </it>and <it>SLA1 </it>that were also identified in the SGA. In contrast, a specific feature of mutant <it>ccw12</it>Δ is the transcriptional repression of genes involved in mating. Physiological experiments substantiate this finding. Further, we demonstrate that Ccw12p is present at the cell periphery and highly concentrated at the presumptive budding site, around the bud, at the septum and at the tip of the mating projection. Conclusions The combination of high throughput screenings, phenotypic analyses and localization studies provides new insight into the function of Ccw12p. A compensatory response, culminating in cell wall remodelling and transport/recycling pathways is required to buffer the loss of <it>CCW12</it>. Moreover, the enrichment of Ccw12p in bud, septum and mating projection is consistent with a role of Ccw12p in preserving cell wall integrity at sites of active growth. The microarray data produced in this analysis have been submitted to NCBI GEO database and GSE22649 record was assigned.</p

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