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AMINO ACID SEQUENCE ANALYSIS OF HUMAN INTERLEUKIN 1
AMINO ACID SEQUENCE ANALYSIS OF HUMAN INTERLEUKIN 1

Cloning and Expression of Bovine Sodium/Glucose Cotransporters* J. Dairy Sci. 88:182–194
Cloning and Expression of Bovine Sodium/Glucose Cotransporters* J. Dairy Sci. 88:182–194

... Rapid Amplification of cDNA Ends and Cloning of bSGLT1 and bSGLT5 The sequences of all primer oligonucleotides used in this study are listed in Table 1. The 3′ and 5′ sequences of bovine solute carrier family 5 (sodium/glucose cotransporter) member 1 and 5 (bSGLT1 and bSGLT5) were obtained by rapid ...
Lecture 3 Isoelectric Focusing
Lecture 3 Isoelectric Focusing

... less -vely charged (pH not so much >pI) (+electrode does not attract protein so much – protein slows down) When reaches the pH 8 region, protein charge =0, -electrode no longer attracts protein, protein stops moving So no matter where the protein is placed, it will move to the region of the gel wher ...
Article - Andrej Sali
Article - Andrej Sali

... the channel are at 8.7 and 24 Å resolution, respectively (Figure S1). A rotation series of the RCC is shown in Figure 1, with the small subunit in gold and the large subunit in blue. Many rods and spiral, ribbon-like features are present on the surface of the ribosome, which can be attributed to ...
Docking with GOLD Tutorial
Docking with GOLD Tutorial

... a docking setup has any chance of success in a drug discovery project. Please download the example folder of input files. Is this an easy docking ? No! You will meet the following challenges:  11 non-trivial rotatable bonds in the ligand  a flexible sugar ring in the ligand  a partially open shap ...
Amino Acid Phylogeny
Amino Acid Phylogeny

... (mutation) of a gene that codes for a protein may result in a change in the amino-acid sequence of the protein. Biochemical evidence of evolution compares favorably with structural evidence of evolution. Even organisms that appear to have few physical similarities may have similar sequences of amino ...
Improved detection and identification of low
Improved detection and identification of low

... over 20 h. IPG strips can also be run on IPGphor™ electrophoresis unit using paper bridges on Cup Loading Strip Holder, which achieves equally high spot resolution. All chemicals and reagents used for the second dimension of 2-D electrophoresis are described in reference 6. Initial equilibration of ...
Representation and High-Quality Annotation of
Representation and High-Quality Annotation of

... amount of data generated during and in the aftermath of large-scale sequencing projects in a user-friendly way is crucial in order to extract biologically meaningful conclusions and hypotheses (Reiser et al., 2002). For most projects, especially in an academic context, an all-in-one solution for the ...
Solubility of recombinant Src homology 2 domains expressed in E
Solubility of recombinant Src homology 2 domains expressed in E

... of beta-aggregation stretches in proteins [13], TANGO (http://tango.crg.es). TANGO analysis of the human TSAd SH2 domain sequence (S90-R188) revealed that the βC strand of the human TSAd SH2 domain (Figure 1) harbours a nine aa sequence (SAVTFVLTY) with near 100% propensity for intermolecular beta-s ...
A new type of plant chitinase containing LysM domains from a fern
A new type of plant chitinase containing LysM domains from a fern

... et al. 1993; Graham and Sticklen 1994). However, an endogenous substrate for plant chitinases has not yet been found. In the absence of an endogenous substrate, plant chitinases may be involved in the interaction between plants and microbes, which produce chitin and chitin-related compounds. One of ...
Safety Assessment of Soy Proteins and Peptides as Used in
Safety Assessment of Soy Proteins and Peptides as Used in

... 71 kDa) and β (ca 50 kDa). The 11S globulin is a hexamer, and is made up of five different subunits, each of which consists of an acidic subunit A (ca 35 kDa) and a basic subunit B (ca 20 kDa), linked by a disulfide bond. The 11S globulin was found to dissociate into 2S, 3S or 7S forms in solutions ...
The Enolase Superfamily: A General Strategy for Enzyme
The Enolase Superfamily: A General Strategy for Enzyme

NATIONAL BOARD OF PODIATRIC MEDICAL EXAMINERS
NATIONAL BOARD OF PODIATRIC MEDICAL EXAMINERS

... include question formats found in the actual examination. They also include questions of varying difficulty. A candidate’s performance on a Practice Test does not guarantee similar performance on the actual examination. ...
Biological significance of structural differences between two highly
Biological significance of structural differences between two highly

... L. Pelzer et al. / Biochemical and Biophysical Research Communications 378 (2009) 563–568 ...
PROTEIN SUBCELLULAR LOCALIZATION
PROTEIN SUBCELLULAR LOCALIZATION

... PSORT are shown in Table 4. For those tables the value of k was optimized separately for the taboo and no taboo list cases. The WoLF PSORT weight vectors (one per partition) however were only trained using the taboo list. The confusion matrices for the WoLF PSORT cross-validation for yeast (which ha ...
A1071 GM Canola MON88302 AppR SD1
A1071 GM Canola MON88302 AppR SD1

... The identity of MON88302-derived CP4 EPSPS was confirmed by a number of analytical techniques, namely recognition by anti-CP4 EPSPS antibody, MALDI-TOF analysis, Nterminal sequencing and enzymatic activity. Bioinformatic studies have confirmed the lack of any significant amino acid sequence similari ...
Document
Document

... • Alignment is simulated as Markov process, all sequence positions are seen as independent • Chances of sequence events are independent – Therefore, probabilities per aligned position need to be multiplied – Amino acid matrices contain so-called log-odds values (log10 of the probabilities), so proba ...
Predicting the sidechain dihedral angle distributions
Predicting the sidechain dihedral angle distributions

... steric, electrostatic, and the attractive component of van der Waals interactions, determine the structure of proteins in general and the conformations of amino acid side chains in particular. However, the relative contributions of the different types of interactions are not known. For example, the ...
PDF of original
PDF of original

... third positions of triplets comprising degenerate codon sets. In all cases triplet pairs with 3'-terminal pyrimidines (XYU and XYC, where X and Y represent the first and second bases, respectively, in the triplet) correspond to the same amino acid; often XYA and XYG correspond to the same amino acid ...
Sequence and Tissue Distribution of a Second Protein of Hepatic
Sequence and Tissue Distribution of a Second Protein of Hepatic

The sequence of human serum albumin cDNA and its expression in
The sequence of human serum albumin cDNA and its expression in

... The mature HSA mRNA sequence was joined to a vector plasmid for direct expression of the mature protein in £ . c o l i via the trp promoter-operator. The plasmid pLelF A25 directs the expression of human leukocyte interferon A (IFNa2) (21). I t was digested with Xbal and the cleavage site " f i l l ...
A structural comparison of molybdenum cofactor
A structural comparison of molybdenum cofactor

... each family, sequence similarities are obvious, while no signi¢cant homologies can be detected between members of di¡erent families. This classi¢cation represents a unifying approach in terms of the overall enzyme structure, but, at the same time, it does not require the Mo/W center to be coordinate ...
Amino Acids
Amino Acids

... • In contrast to globular proteins, whose shapes result from complex interactions b/w 2º, 3º, and sometimes 4º ...
High pKa variability of cysteine residues in structural databases and
High pKa variability of cysteine residues in structural databases and

... For our benchmark, we selected a set of proteins from literature; because of limited experimental information, Cys is often avoided in protein pKa benchmarks [17,23]. To collect reference information we have looked for publications reporting experimentally derived Cys pKa; among them, we searched fo ...
r Functional perspectives on the evolution of argasid tick
r Functional perspectives on the evolution of argasid tick

... 2.3.9 The influence of savignygrin on platelet shape change 2.3.10 Targeting of allb~3 by savignygrin 2.3.1 1 Integrin specificity of savignygrin 2.3.12 N-terminal amino acid sequence determination of the savignygrins 2.3.13 Isolation of total RNA 2.3.14 Cloning and sequencing of savignygrin 2.3.15 ...
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Homology modeling



Homology modeling, also known as comparative modeling of protein, refers to constructing an atomic-resolution model of the ""target"" protein from its amino acid sequence and an experimental three-dimensional structure of a related homologous protein (the ""template""). Homology modeling relies on the identification of one or more known protein structures likely to resemble the structure of the query sequence, and on the production of an alignment that maps residues in the query sequence to residues in the template sequence. It has been shown that protein structures are more conserved than protein sequences amongst homologues, but sequences falling below a 20% sequence identity can have very different structure.Evolutionarily related proteins have similar sequences and naturally occurring homologous proteins have similar protein structure.It has been shown that three-dimensional protein structure is evolutionarily more conserved than would be expected on the basis of sequence conservation alone.The sequence alignment and template structure are then used to produce a structural model of the target. Because protein structures are more conserved than DNA sequences, detectable levels of sequence similarity usually imply significant structural similarity.The quality of the homology model is dependent on the quality of the sequence alignment and template structure. The approach can be complicated by the presence of alignment gaps (commonly called indels) that indicate a structural region present in the target but not in the template, and by structure gaps in the template that arise from poor resolution in the experimental procedure (usually X-ray crystallography) used to solve the structure. Model quality declines with decreasing sequence identity; a typical model has ~1–2 Å root mean square deviation between the matched Cα atoms at 70% sequence identity but only 2–4 Å agreement at 25% sequence identity. However, the errors are significantly higher in the loop regions, where the amino acid sequences of the target and template proteins may be completely different.Regions of the model that were constructed without a template, usually by loop modeling, are generally much less accurate than the rest of the model. Errors in side chain packing and position also increase with decreasing identity, and variations in these packing configurations have been suggested as a major reason for poor model quality at low identity. Taken together, these various atomic-position errors are significant and impede the use of homology models for purposes that require atomic-resolution data, such as drug design and protein–protein interaction predictions; even the quaternary structure of a protein may be difficult to predict from homology models of its subunit(s). Nevertheless, homology models can be useful in reaching qualitative conclusions about the biochemistry of the query sequence, especially in formulating hypotheses about why certain residues are conserved, which may in turn lead to experiments to test those hypotheses. For example, the spatial arrangement of conserved residues may suggest whether a particular residue is conserved to stabilize the folding, to participate in binding some small molecule, or to foster association with another protein or nucleic acid. Homology modeling can produce high-quality structural models when the target and template are closely related, which has inspired the formation of a structural genomics consortium dedicated to the production of representative experimental structures for all classes of protein folds. The chief inaccuracies in homology modeling, which worsen with lower sequence identity, derive from errors in the initial sequence alignment and from improper template selection. Like other methods of structure prediction, current practice in homology modeling is assessed in a biennial large-scale experiment known as the Critical Assessment of Techniques for Protein Structure Prediction, or CASP.
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