Computational studies of protein posttranslational modification : glycosylation of oligoproline and collagen peptides

xvi, 238 leaves : ill. ; 29 cmGlycosylation is the most complex posttranslational modification of proteins and has consequences on protein structure and function. In particular, the hydroxyproline (Hyp) rich glycoproteins (HRGPs) of plants are heavily glycosylated. On the other hand, glycosylation has not been observed in animal collagen despite the high occurrence of Hyp residues. This thesis uses computational chemistry to provide molecular level information about the structural effects of Hyp glycosylation to help understand the biological implications of the modification and explain the lack of glycosylation in animals. Initially, the nature of the glycosidic linkage between Hyp and galactose was determined. The theoretical results were validated by comparing to the recent experimental data, which helped understand other experimental observations. Subsequently, contiguous and non-contiguous glycosylation of a nonaproline oligopeptide was considered, which revealed that contiguous glycosylation increases the stability of the all trans polyproline II (PPII) conformation, while non-contiguous glycosylation leads to loss of PPII content. Sophisticated modeling suggested that this difference arises since peptide–solvent interactions stabilize the PPII conformation in the contiguously glycosylated peptide, while sugar–peptide backbone interactions that stabilize the cis conformations of some residues are stronger in the non-contiguously glycosylated peptide. Finally, the effects of Hyp glycosylation on the collagen triple helix were assessed, where it was determined that glycosylation makes the monomeric state more stable and hence hinders triple helix formation, which agrees with experimental results and highlights that the synergy between computation and experiments is necessary to understand complex glycosylation in nature

Computational Studies of Glycan Conformations in Glycoproteins

N-glycans refer to oligosaccharide chains covalently attached to the side chain of asparagine (Asn) residues, and the majority of proteins synthesized in the endoplasmic reticulum (ER) are N-glycosylated. N-glycans can modulate the structural properties of proteins due to their close proximity to their parent proteins and their interactions between the glycan and the protein surface residues. In addition, N-glycans provide specific regions of recognition for cellular and molecular recognition. Despite their biological importance, the structural understanding of glycans and the impact of glycosylation to glycan or protein structure are lacking. I have explored the conformational freedom of glycans and their conformational preferences in different environments using structural databases and computer simulations. First, I have developed an algorithm to reliably annotate a given atomic structure of glycans. This algorithm is important because many glycan molecules in the crystal structure database are misannotated or contain errors. Using the algorithm, a database of glycans found in the PDB is constructed and available to the public. Second, the impact of glycosylation on the glycan conformation has been examined. Contrary to the common belief that the glycan conformations are independent to the protein structure, it appears that the protein structure can significantly affect the glycan structure upon glycosylation. This observation is significant because it may provide insight into protein-glycan interaction and opens up the possibility of a template-based glycan modeling approach. Third, the differences in conformational preference between glycans in solution and in glycoproteins has been examined. Using molecular dynamics (MD) simulations, the conformational preference of N-glycan pentassacharide in solution is exhaustively studied. Surprisingly, the conformational distribution is dominated by a single major conformational state and several minor conformational states. The dominant conformational state adopts a more extended conformation, thus it appears that entropy plays an important role in determining the conformational state. On the other hand, in glycoproteins, glycans can interact with surrounding protein side chains and, as a result, several conformational states are more equally populated. Based on these observations, a protocol is proposed for modeling the glycan portion of a known protein structure. It is typically more managable to acquire an atomic resolution structure or aglycoprotein (glycoprotein without glycan). In addition, the glycoform and the glycosylation site can be identified independently by mass spectrometry or NMR. The proposed modeling protocol assumes the glycosylation site, glycoform, and aglycoprotein structure are already known, and builds glycan structure models on top of the known aglycoprotein structure. The performance of the modeling protocol is greatly improved by using appropriate template structures. This protocol can be used to generate the initial model for MD simulations or refinement of low resolution models from experiments (small angle X-ray scattering and electron microscopy)

Biomolecular recognition mechanisms studied by NMR spectroscopy and MD simulations

This thesis describes the use of solution Nuclear Magnetic Resonance (NMR) spectroscopy and Molecular Dynamics (MD) simulations to study the mechanism of biomolecular recognition with two model systems: i) lipid II-binding lantibiotics (lanthionine-containing antibiotics) and ii) the human immunodeficiency virus 1 (HIV-1) envelope protein (Env), gp120, and its receptor molecule, CD4. The first system concerns a group of unique antimicrobial peptides, which make use of an hitherto unknown mechanism of attacking bacteria by targeting the Achilles¹ heel of bacteria, the cell wall precursor, lipid II. In the light of antibiotic resistance, understanding of this recognition mechanism may lead to novel antibiotics. The second system focuses on the initiation step of the HIV-1 viral entry wherein the engagement of gp120 and CD4 switches on a cascade of conformational changes that are necessary for the membrane fusion between the virus and the host cell. The biological contexts of both systems are important to human health and numerous functional studies on both systems have been well documented. Yet, because of the underlying dynamics and the intricate assembly process of higher order complexes, a detailed structural description is currently lacking in both systems. We therefore applied advanced NMR and MD techniques to unravel the structure and dynamics of these complexes with the hope to facilitate the development of new antibiotics and vaccines for infectious diseases, such as AIDS. As biological functions are manifested by interactions at a molecular level, understanding of structural properties of these biomolecules may consolidate related biomedical research

Psr1p interacts with SUN/sad1p and EB1/mal3p to establish the bipolar spindle

Regular Abstracts - Sunday Poster Presentations: no. 382During mitosis, interpolar microtubules from two spindle pole bodies (SPBs) interdigitate to create an antiparallel microtubule array for accommodating numerous regulatory proteins. Among these proteins, the kinesin-5 cut7p/Eg5 is the key player responsible for sliding apart antiparallel microtubules and thus helps in establishing the bipolar spindle. At the onset of mitosis, two SPBs are adjacent to one another with most microtubules running nearly parallel toward the nuclear envelope, creating an unfavorable microtubule configuration for the kinesin-5 kinesins. Therefore, how the cell organizes the antiparallel microtubule array in the first place at mitotic onset remains enigmatic. Here, we show that a novel protein psrp1p localizes to the SPB and plays a key role in organizing the antiparallel microtubule array. The absence of psr1+ leads to a transient monopolar spindle and massive chromosome loss. Further functional characterization demonstrates that psr1p is recruited to the SPB through interaction with the conserved SUN protein sad1p and that psr1p physically interacts with the conserved microtubule plus tip protein mal3p/EB1. These results suggest a model that psr1p serves as a linking protein between sad1p/SUN and mal3p/EB1 to allow microtubule plus ends to be coupled to the SPBs for organization of an antiparallel microtubule array. Thus, we conclude that psr1p is involved in organizing the antiparallel microtubule array in the first place at mitosis onset by interaction with SUN/sad1p and EB1/mal3p, thereby establishing the bipolar spindle.postprin

Removal of antagonistic spindle forces can rescue metaphase spindle length and reduce chromosome segregation defects

Regular Abstracts - Tuesday Poster Presentations: no. 1925Metaphase describes a phase of mitosis where chromosomes are attached and oriented on the bipolar spindle for subsequent segregation at anaphase. In diverse cell types, the metaphase spindle is maintained at a relatively constant length. Metaphase spindle length is proposed to be regulated by a balance of pushing and pulling forces generated by distinct sets of spindle microtubules and their interactions with motors and microtubule-associated proteins (MAPs). Spindle length appears important for chromosome segregation fidelity, as cells with shorter or longer than normal metaphase spindles, generated through deletion or inhibition of individual mitotic motors or MAPs, showed chromosome segregation defects. To test the force balance model of spindle length control and its effect on chromosome segregation, we applied fast microfluidic temperature-control with live-cell imaging to monitor the effect of switching off different combinations of antagonistic forces in the fission yeast metaphase spindle. We show that spindle midzone proteins kinesin-5 cut7p and microtubule bundler ase1p contribute to outward pushing forces, and spindle kinetochore proteins kinesin-8 klp5/6p and dam1p contribute to inward pulling forces. Removing these proteins individually led to aberrant metaphase spindle length and chromosome segregation defects. Removing these proteins in antagonistic combination rescued the defective spindle length and, in some combinations, also partially rescued chromosome segregation defects. Our results stress the importance of proper chromosome-to-microtubule attachment over spindle length regulation for proper chromosome segregation.postprin

Marine Proteins and Peptides

Marine proteins and peptides have great potential application in developing pharmaceuticals, nutraceuticals, and cosmeceuticals. Proteins and peptides from marine sources are considered to be safe and inexpensive. Protein- and peptide-based drugs have been increasing in recent days to cure various diseases by serving multiple roles, such as antioxidants, anticancer drugs, antimicrobials, and anticoagulants. There are different marine sources (macroalgae, fish, shellfish, and bivalves), which possibly contain specific protein and peptides

Non-covalent interactions in organotin(IV) derivatives of 5,7-ditertbutyl- and 5,7-diphenyl-1,2,4-triazolo[1,5-a]pyrimidine as recognition motifs in crystalline self- assembly and their in vitro antistaphylococcal activity

Non-covalent interactions are known to play a key role in biological compounds due to their stabilization of the tertiary and quaternary structure of proteins [1]. Ligands similar to purine rings, such as triazolo pyrimidine ones, are very versatile in their interactions with metals and can act as model systems for natural bio-inorganic compounds [2]. A considerable series (twelve novel compounds are reported) of 5,7-ditertbutyl-1,2,4-triazolo[1,5-a]pyrimidine (dbtp) and 5,7-diphenyl- 1,2,4-triazolo[1,5-a]pyrimidine (dptp) were synthesized and investigated by FT-IR and 119Sn M\uf6ssbauer in the solid state and by 1H and 13C NMR spectroscopy, in solution [3]. The X-ray crystal and molecular structures of Et2SnCl2(dbtp)2 and Ph2SnCl2(EtOH)2(dptp)2 were described, in this latter pyrimidine molecules are not directly bound to the metal center but strictly H-bonded, through N(3), to the -OH group of the ethanol moieties. The network of hydrogen bonding and aromatic interactions involving pyrimidine and phenyl rings in both complexes drives their self-assembly. Noncovalent interactions involving aromatic rings are key processes in both chemical and biological recognition, contributing to overall complex stability and forming recognition motifs. It is noteworthy that in Ph2SnCl2(EtOH)2(dptp)2 \u3c0\u2013\u3c0 stacking interactions between pairs of antiparallel triazolopyrimidine rings mimick basepair interactions physiologically occurring in DNA (Fig.1). M\uf6ssbauer spectra suggest for Et2SnCl2(dbtp)2 a distorted octahedral structure, with C-Sn-C bond angles lower than 180\ub0. The estimated angle for Et2SnCl2(dbtp)2 is virtually identical to that determined by X-ray diffraction. Ph2SnCl2(EtOH)2(dptp)2 is characterized by an essentially linear C-Sn-C fragment according to the X-ray all-trans structure. The compounds were screened for their in vitro antibacterial activity on a group of reference staphylococcal strains susceptible or resistant to methicillin and against two reference Gramnegative pathogens [4] . We tested the biological activity of all the specimen against a group of staphylococcal reference strains (S. aureus ATCC 25923, S. aureus ATCC 29213, methicillin resistant S. aureus 43866 and S. epidermidis RP62A) along with Gram-negative pathogens (P. aeruginosa ATCC9027 and E. coli ATCC25922). Ph2SnCl2(EtOH)2(dptp)2 showed good antibacterial activity with a MIC value of 5 \u3bcg mL-1 against S. aureus ATCC29213 and also resulted active against methicillin resistant S. epidermidis RP62A