Critical assessment of predicted interactions at atomic resolution

Mendez Giraldez, Raul

21 September 2007

Molecular Biology has allowed the characterization and manipulation of the molecules of life in the wet lab. Also the structures of those macromolecules are being continuously elucidated. During the last decades of the past century, there was an increasing interest to study how the different genes are organized into different organisms (‘genomes’) and how those genes are expressed into proteins to achieve their functions. Currently the sequences for many genes over several genomes have been determined. In parallel, the efforts to have the structure of the proteins coded by those genes go on. However it is experimentally much harder to obtain the structure of a protein, rather than just its sequence. For this reason, the number of protein structures available in databases is an order of magnitude or so lower than protein sequences. Furthermore, in order to understand how living organisms work at molecular level we need the information about the interaction of those proteins. Elucidating the structure of protein macromolecular assemblies is still more difficult. To that end, the use of computers to predict the structure of these complexes has gained interest over the last decades.<p>The main subject of this thesis is the evaluation of current available computational methods to predict protein – protein interactions and build an atomic model of the complex. The core of the thesis is the evaluation protocol I have developed at Service de Conformation des Macromolécules Biologiques et de Bioinformatique, Université Libre de Bruxelles, and its computer implementation. This method has been massively used to evaluate the results on blind protein – protein interaction prediction in the context of the world-wide experiment CAPRI, which have been thoroughly reviewed in several publications [1-3]. In this experiment the structure of a protein complex (‘the target’) had to be modeled starting from the coordinates of the isolated molecules, prior to the release of the structure of the complex (this is commonly referred as ‘docking’).<p>The assessment protocol let us compute some parameters to rank docking models according to their quality, into 3 main categories: ‘Highly Accurate’, ‘Medium Accurate’, ‘Acceptable’ and ‘Incorrect’. The efficiency of our evaluation and ranking is clearly shown, even for borderline cases between categories. The correlation of the ranking parameters is analyzed further. In the same section where the evaluation protocol is presented, the ranking participants give to their predictions is also studied, since often, good solutions are not easily recognized among the pool of computer generated decoys.<p>An overview of the CAPRI results made per target structure and per participant regarding the computational method they used and the difficulty of the complex. Also in CAPRI there is a new ongoing experiment about scoring previously and anonymously generated models by other participants (the ‘Scoring’ experiment). Its promising results are also analyzed, in respect of the original CAPRI experiment. The Scoring experiment was a step towards the use of combine methods to predict the structure of protein – protein complexes. We discuss here its possible application to predict the structure of protein complexes, from a clustering study on the different results.<p>In the last chapter of the thesis, I present the preliminary results of an ongoing study on the conformational changes in protein structures upon complexation, as those rearrangements pose serious limitations to current computational methods predicting the structure protein complexes. Protein structures are classified according to the magnitude of its conformational re-arrangement and the involvement of interfaces and particular secondary structure elements is discussed. At the end of the chapter, some guidelines and future work is proposed to complete the survey. / Doctorat en Sciences / info:eu-repo/semantics/nonPublished

Sciences exactes et naturelles

Chimie

Structural bioinformatics

Molecular structure

Proteins -- Conformation

Proteins -- Structure

Amino acids

Bio-informatique structurale

Structure moléculaire

Protéines -- Conformation

Protéines -- Structure

Acides aminés

protein - protein complex

protein - protein interaction

root mean square deviation

docking

solvent accessible area

conformational change

rmsd

Electrostaticanalisys the Ras active site

Khan, Abdul Kareem

05 March 2009

La preorganització electrostàtica del centre actiu s'ha postulat com el mecanisme genèric de l'acció dels enzims. Així, alguns residus "estratègics" es disposarien per catalitzar reaccions interaccionant en una forma més forta amb l'estat de transició, baixant d'aquesta manera el valor de l'energia dactivació &#61508;g cat. S'ha proposat que aquesta preorientació electrostática s'hauria de poder mostrar analitzant l'estabilitat electrostàtica de residus individuals en el centre actiu.Ras es una proteïna essencial de senyalització i actúa com un interruptor cel.lular. Les característiques estructurals de Ras en el seu estat actiu (ON) són diferents de les que té a l'estat inactiu (OFF). En aquesta tesi es duu a terme una anàlisi exhaustiva de l'estabilitat dels residus del centre actiu deRas en l'estat actiu i inactiu. / The electrostatic preorganization of the active site has been put forward as the general framework of action of enzymes. Thus, enzymes would position "strategic" residues in such a way to be prepared to catalyze reactions byinteracting in a stronger way with the transition state, in this way decreasing the activation energy &#61508;g cat for the catalytic process. It has been proposed thatsuch electrostatic preorientation should be shown by analyzing the electrostatic stability of individual residues in the active site.Ras protein is an essential signaling molecule and functions as a switch in thecell. The structural features of the Ras protein in its active state (ON state) are different than those in its inactive state (OFF state). In this thesis, an exhaustive analysis of the stability of residues in the active and inactive Ras active site is performed.

dinàmica

centre actiu

relacions d'estructura activitat

preorganització

reorganització

estat de transició

estat actiu

estabilitat electrostàtica

interacción proteïna-proteïna

test de ranks de Wilcoxon

P-loop

G1 motif

HVR

metastability

RMSD

substrate assisted catalysis

sequence alignment

beta sheet

helix

Z-test

wilcoxon rank test

protein-protein interactions

electrostatic stability

active state

dynamics

signal transduction

electrostatic stabilization

ras effectors

guanine exchange factor

GTPase-activating proteins

quantum mechanics/molecular

PDLD/S-LRA

X-ray crystallography

solvation energy

free energy perturbation

statistical analysis

GTP hydrolysis

guanosine diphosphate

guanosine triphosphate

computer simulation

thermodynamics

protein conformation

electrostatics

interruptor II

interruptor I

llaç P

motiu G1

HVR (regions altament variables)

metaestabilita

RMSD

catàlisi assistida pel substrat

aliniament de seqüència

fulla beta

hèlix

test Z

transducció del senyal

estabilització electrostàtica

efectors de ras

factor de bescamvi de guanina

proteïnes activadores de l'activitat

mecànica quàntica/mecànica

PDLD/S-LRA

cristalografia de raigs X

energia de solvatació

perturbació de l'energia lliure

anàlisi estadística

hidròlisi de GTP

difosfat de guanosina

trifosfat de guanosina

simulació computacional

termodinàmica

conformació proteïca

electrostàtica

switch-I

switch-II

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