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level: Level 1 of L11.Protein Structure Analysis

Questions and Answers List

level questions: Level 1 of L11.Protein Structure Analysis

QuestionAnswer
what are protein functions determined by? what are the folds determined by?• Protein functions are determined by their structures. • Essential elements in bioinformatics. • Conformation (folding) of protein is determined by dihedral angle (phi and psi).
what are amino acids linked byAmino acids are linked by peptide bond.
how are the ψ (psi) against φ (phi) angles visualized?Ramachandran plot visualizes backbone dihedral angles ψ (psi) against φ (phi) of amino acid residues in protein structure.
what's the difference between protein Structure Analysis and Prediction ?-protein structure analysis - usually refers to the determination of the protein structure by physical or chemical methods. -Protein structure prediction - refers to the inference of the protein structure using computer algorithms
what are the four different protein structures?1-Primary Structure – Sequence of amino acids 2-Secondary Structure – Local Structure such as a-helices and b-sheet. 3-tertiary Structure –Arrangement of the secondary structural elements to give 3- dimensional structure of a protein. 4- Quaternary Structure– Arrangement of the subunits to give a protein complex its 3- dimensional structure.
how are protein structures determined ?• X-ray crystallography • NMR spectroscopy • Cryo-electron microscopy • Neutron diffraction • Atomic force microscopy
what is used to measure protein structure?X-ray diffraction analysis – must first be able to crystallize the protein and then calculate its structure by the way it disperses X-rays. determining the protein structure directly is difficult.
how does X-ray crystallography work ? what is used to determine quality?– Protein need to be grown into large crystal – The X-ray are reflected by electron cloud surrounding the atoms, diffraction patterns are converted into electron density map. The quality is determined by -R factor is used to determined the quality of the model, ranging from 0.0 – 0.59
what are the two methods used in X-ray crystallography to resolve the structures?• Molecular replacement • Multiple isomorphous replacement
what are the steps going from x-ray got atomic model?N
how does NMR (Nuclear Magnetic Resonance) work ?– Detect spinning pattern of atomic nuclei in magnetic field – Protein are in solution, so it is mobile and vibrating, thus a number of different models will be constructed. – Limit to <200 amino acid residues, use radioisotope
what are the limitations of both X-rayDiffraction and NMRDistanceMeasurement?• X-rayDiffraction ✓ Only a small number of proteins can be made to form crystals ✓ A crystal is not the protein’s native environment ✓ Very time consuming • NMRDistanceMeasurement ✓ Not all proteins are found in solution ✓ This method generally looks at isolated proteins rather than protein complexes ✓ Very time consuming
how are structures verified and validated?•MolProbity •NQ-Flipper •Procheck •CheckMyMetal •Prosa-web •Uppsala Electron Density Server •Verify3D Structure Evaluation Server •WHAT_CHECK •WHAT IF
how does a Ramachandran Plot look like?N
what's Cryo-electron microscopy?• Transmission EM at very low temperatures (liquid nitrogen) • Veryhighresolution(3-4Å)
what's Atomic force microscopy?• Type of Scanning Probe Microscopy (SPM) • Invented in 1985 by IBM • Provides resolution of a fraction of a nanometer
what's Structure-structure alignment and comparison?its done by placing them side by side and comparing them.
how are conformational changes analyzed ?there are two forms open form and closed form . Citrate synthase, ligand induced conformational changes Domain motion and small structural distortions.
why do we Defining Domains?Link between domain structure and function -Different structural domains can be associated with different functions. -Enzyme active sites are often at domain interfaces; domain movements play a functional role.
what are the Methods for Identifying Domains?Domain limits are defined by identifying groups of residues such that the number of contacts between groups is minimized.