Importance of the two tryptophan residues in the Streptomyces R61 exocellular dd-peptidase

Modification of the Streptomyces R61 DD-peptidase by N-bromosuccinimide resulted in a rapid loss of enzyme activity. In consequence, the role of the enzyme's two tryptophan residues was investigated by site-directed mutagenesis. Trp271 was replaced by Leu. The modification yielded a stable enzyme whose structural and catalytic properties were similar to those of the wild-type protein. Thus the Trp271 residue, though almost invariant among the beta-lactamases of classes A and C and the low-Mr penicillin-binding proteins, did not appear to be essential for enzyme activity. Mutations of the Trp233 into Leu and Ser strongly decreased the enzymic activity, the affinity for beta-lactams and the protein stability. Surprisingly, the benzylpenicilloyl-(W233L)enzyme deacylated at least 300-fold more quickly than the corresponding acyl-enzyme formed with the wild-type protein and gave rise to benzylpenicilloate instead of phenylacetylglycine. This mutant DD-peptidase thus behaved as a weak beta-lactamase.

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Expression of the Schwanniomyces occidentalis SWA2 amylase in Saccharomyces cerevisiae: role of N-glycosylation on activity, stability and secretion

Biochemical Journal ◽

10.1042/bj3290065 ◽

1998 ◽

Vol 329 (1) ◽

pp. 65-71 ◽

Cited By ~ 36

Author(s):

Esther YÁÑEZ ◽

A. Teresa CARMONA ◽

Mercedes TIEMBLO ◽

Antonio JIMÉNEZ ◽

María FERNÁNDEZ-LOBATO

Keyword(s):

Saccharomyces Cerevisiae ◽

Catalytic Efficiency ◽

Extracellular Enzyme ◽

Site Directed Mutagenesis ◽

Activity Levels ◽

Wild Type ◽

Schwanniomyces Occidentalis ◽

Type Protein ◽

Wild Type Protein

The role of N-linked glycosylation on the biological activity of Schwanniomyces occidentalis SWA2 α-amylase, as expressed in Saccharomyces cerevisiae, was analysed by site-directed mutagenesis of the two potential N-glycosylation sites, Asn-134 and Asn-229. These residues were replaced by Ala or Gly individually or in various combinations and the effects on the activity, secretion and thermal stability of the enzyme were studied. Any Asn-229 substitution caused a drastic decrease in activity levels of the extracellular enzyme. In contrast, substitutions of Asn-134 had little or no effect. The use of antibodies showed that α-amylase was secreted in all the mutants tested, although those containing substitutions at Asn-229 seemed to have a lower rate of synthesis and/or higher degradation than the wild-type strain. α-Amylases with substitution at Asn-229 had a 2 kDa lower molecular mass than the wild-type protein, as did the wild-type protein itself after treatment with endoglycosidase F. These findings indicate that Asn-229 is the single glycosylated residue in SWA2. Thermostability analysis of both purified wild-type (T50 = 50 °C, where T50 is the temperature resulting in 50% loss of activity) and mutant enzymes indicated that removal of carbohydrate from the 229 position results in a decrease of approx. 3 °C in the T50 of the enzyme. The Gly-229 mutation does not change the apparent affinity of the enzyme for starch (Km) but decreases to 1/22 its apparent catalytic efficiency (kcat/Km). These results therefore indicate that glycosylation at the 229 position has an important role in the extracellular activity levels, kinetics and stability of the Sw. occidentalis SWA2 α-amylase in both its wild-type and mutant forms.

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Revisiting the role of PML protein targeting and disruption of PML bodies in human cytomegalovirus infection

Access Microbiology ◽

10.1099/acmi.ac2020.po0734 ◽

2020 ◽

Vol 2 (7A) ◽

Author(s):

Christina Paulus ◽

Thomas Harwardt ◽

Bernadette Walter ◽

Andrea Marxreiter ◽

Michael Nevels

Keyword(s):

Gene Expression ◽

Viral Replication ◽

Human Cytomegalovirus ◽

Critical Role ◽

Wild Type ◽

Early Protein ◽

Type Protein ◽

Wild Type Protein ◽

Pml Bodies

Promyelocytic leukaemia (PML) bodies are nuclear organelles implicated in post-translational modification by small ubiquitin-like modifier (SUMO) proteins and in the antiviral host cell response to infection. The 72-kDa immediate-early protein 1 (IE1) is considered the principal antagonist of PML bodies encoded by the human cytomegalovirus, one of eight human herpesviruses. Previous work has suggested that the interaction between IE1 and PML proteins, the central organisers of PML bodies, and the subsequent disruption of these organelles serve a critical role in viral replication by counteracting intrinsic antiviral immunity and the induction of interferon (IFN)-stimulated genes. However, this picture has emerged largely from studying mutant IE1 proteins known or predicted to be globally misfolded und metabolically unstable. We systematically screened for stable IE1 mutants by clustered charge-to-alanine scanning. We identified a mutant protein (IE1cc172-176) selectively defective for PML interaction. Functional comparisons between the mutant and wild-type protein revealed that IE1 can undergo modification by mixed polymeric SUMO chains and that it targets PML and Sp100, the two main constituents of PML bodies, via distinct mechanisms. Unexpectedly, IE1cc172-176 supported viral replication almost as efficiently as wild-type IE1. Moreover, lower instead of higher (as expected) levels of tumor necrosis factor alpha, IFN-beta, IFN-lambda and IFN-stimulated gene expression were observed with the mutant compared to the wild-type protein and virus. These results suggest that the disruption of PML bodies is linked to induction rather than inhibition of antiviral gene expression. Our findings challenge current views regarding the role of PML bodies in viral infection.

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Loss of enzyme activity in a site-directed mutant of influenza neuraminidase compared to expressed wild-type protein

Virology ◽

10.1016/0042-6822(86)90404-6 ◽

1986 ◽

Vol 148 (1) ◽

pp. 74-83 ◽

Cited By ~ 17

Author(s):

Michael R. Lentz ◽

Gillian M. Air

Keyword(s):

Enzyme Activity ◽

Wild Type ◽

Type Protein ◽

Wild Type Protein ◽

A Site

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Role of tryptophan 135 of Chandipura virus phosphoprotein P in dimerization and complex formation with leader RNA: structural aspect using time resolved anisotropy and simulation

RSC Advances ◽

10.1039/c5ra20863g ◽

2015 ◽

Vol 5 (126) ◽

pp. 104582-104593

Author(s):

Manini Mukherjee ◽

Aditya Sarkar ◽

Arunava Roy ◽

Pinki Saha Sardar ◽

Ansuman Lahiri ◽

...

Keyword(s):

Molecular Dynamics ◽

Structural Change ◽

Complex Formation ◽

Protein Concentration ◽

Structural Aspect ◽

Wild Type ◽

Time Resolved ◽

Type Protein ◽

Wild Type Protein

The nanosecond and picosecond dynamics of wild type protein and its tryptophan mutants have been used to study structural change as a function of protein concentration and binding with leader RNA by time resolved anisotropy and molecular dynamics.

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A model system for studying membrane biogenesis. Overexpression of cytochrome b5 in yeast results in marked proliferation of the intracellular membrane

Journal of Cell Science ◽

10.1242/jcs.106.1.249 ◽

1993 ◽

Vol 106 (1) ◽

pp. 249-259 ◽

Cited By ~ 2

Author(s):

G. Vergeres ◽

T.S. Yen ◽

J. Aggeler ◽

J. Lausier ◽

L. Waskell

Keyword(s):

Cytochrome B5 ◽

Alpha Helix ◽

Site Directed Mutagenesis ◽

Directed Mutagenesis ◽

Membrane Biogenesis ◽

Wild Type ◽

Membrane Anchor ◽

Type Protein ◽

Wild Type Protein ◽

Membrane Bound

Cytochrome b5 is an amphipathic microsomal protein that is anchored to the endoplasmic reticulum by a single hydrophobic transmembrane alpha-helix located near the carboxyl terminus of the protein. In yeast, cytochrome b5 provides electrons for fatty acid desaturation and ergosterol biosynthesis. High level expression of cytochrome b5 in Saccharomyces cerevisiae was achieved using the yeast metallothionein promoter and a synthetic cytochrome b5 gene. In order to accommodate the markedly increased amount of the membrane-bound cytochrome b5, the yeast cell proliferated its nuclear membrane. As many as 20 pairs of stacked membranes could be observed to partially encircle the nucleus. This morphological arrangement of membrane around the nucleus is known as a karmella. In an effort to understand which part of the cytochrome b5 molecule, i.e. the membrane anchor or the soluble heme domain, which is competent in electron transfer, provided the signal for the de novo membrane biogenesis, a series of studies, including site-directed mutagenesis, was undertaken. The results of these experiments demonstrated that the inactive hemedeficient apo form of the membrane-bound protein stimulates membrane proliferation to the same extent as the holo wild-type protein, whereas cytosolic forms of cytochrome b5 did not induce membrane synthesis. These data demonstrate that membrane proliferation is a consequence of the cell's ability to monitor the level of membrane proteins and to compensate for alterations in these levels rather than the result of the ability of the extra cytochrome b5 to catalyze synthesis of extra lipid that had to be accommodated in new membrane. Site-directed mutagenesis studies of the membrane binding domain of cytochrome b5 provided additional clues about the nature of the signal for membrane proliferation. Replacement of the membrane anchor by a non-physiological nonsense sequence of 22 leucines gave rise to a mutant protein that triggered membrane biosynthesis. The conclusion from these experiments is clear; the signal for membrane proliferation does not reside in some specific amino acid sequence but instead in the hydrophobic properties of the proliferant. Interestingly, these membranes are somewhat diminished in quantity and have a slightly altered morphology compared to those induced by the wild-type protein. It was also observed that disruption of the putative alpha helix of the membrane anchor by an Ala116Pro mutation, which gives rise to two sequential prolines at positions 115 and 116 results in a protein with diminished capacity to induce membrane formation.(ABSTRACT TRUNCATED AT 400 WORDS)

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The Griffithsin Dimer Is Required for High-Potency Inhibition of HIV-1: Evidence for Manipulation of the Structure of gp120 as Part of the Griffithsin Dimer Mechanism

Antimicrobial Agents and Chemotherapy ◽

10.1128/aac.00332-13 ◽

2013 ◽

Vol 57 (8) ◽

pp. 3976-3989 ◽

Cited By ~ 24

Author(s):

Jie Xue ◽

Bart Hoorelbeke ◽

Ioannis Kagiampakis ◽

Borries Demeler ◽

Jan Balzarini ◽

...

Keyword(s):

Protein A ◽

Carbohydrate Binding ◽

Wild Type ◽

Subtype C ◽

Subtype B ◽

Type Protein ◽

Wild Type Protein ◽

Protein Dimer ◽

Anti Hiv

ABSTRACTGriffithsin (Grft) is a protein lectin derived from red algae that tightly binds the HIV envelope protein gp120 and effectively inhibits virus infection. This inhibition is due to the binding by Grft of high-mannose saccharides on the surface of gp120. Grft has been shown to be a tight dimer, but the role of the dimer in Grft's anti-HIV function has not been fully explored. To investigate the role of the Grft dimer in anti-HIV function, an obligate dimer of Grft was designed by expressing the protein with a peptide linker between the two subunits. This “Grft-linker-Grft” is a folded protein dimer, apparently nearly identical in structural properties to the wild-type protein. A “one-armed” obligate dimer was also designed (Grft-linker-Grft OneArm), with each of the three carbohydrate binding sites of one subunit mutated while the other subunit remained intact. While both constructed dimers retained the ability to bind gp120 and the viral surface, Grft-linker-Grft OneArm was 84- to 1,010-fold less able to inhibit HIV than wild-type Grft, while Grft-linker-Grft had near-wild-type antiviral potency. Furthermore, while the wild-type protein demonstrated the ability to alter the structure of gp120 by exposing the CD4 binding site, Grft-linker-Grft OneArm largely lost this ability. In experiments to investigate gp120 shedding, it was found that Grft has different effects on gp120 shedding for strains from subtype B and subtype C, and this might correlate with Grft function. Evidence is provided that the dimer form of Grft is critical to the function of this protein in HIV inhibition.

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Mechanism of action of dd-peptidases: role of asparagine-161 in the Streptomyces R61 dd-peptidase

Biochemical Journal ◽

10.1042/bj2930195 ◽

1993 ◽

Vol 293 (1) ◽

pp. 195-201 ◽

Cited By ~ 10

Author(s):

J M Wilkin ◽

M Jamin ◽

B Joris ◽

J M Frere

Keyword(s):

Site Directed Mutagenesis ◽

Beta Lactamase ◽

Wild Type ◽

Peptide Substrate ◽

Beta Lactam ◽

Beta Lactams ◽

Wild Type Enzyme ◽

Class A ◽

First Case

The role of residue Asn-161 in the interaction between the Streptomyces R61 DD-peptidase and various substrates or beta-lactam inactivators was probed by site-directed mutagenesis. The residue was successively replaced by serine and alanine. In the first case, acylation rates were mainly affected with the peptide and ester substrates but not with the thiol-ester substrates and beta-lactams. However, the deacylation rates were decreased 10-30-fold with the substrates yielding benzoylglycyl and benzoylalanyl adducts. The Asn161Ala mutant was more generally affected, although the acylation rates with cefuroxime and cefotaxime remained similar to those observed with the wild-type enzyme. Surprisingly, the deacylation rates of the benzoylglycyl and benzoylalanyl adducts were very close to those observed with the wild-type enzyme. The results also indicate that the interaction with the peptide substrate and the transpeptidation reaction were more sensitive to the mutations than the other reactions studied. The results are discussed and compared with those obtained with the Asn-132 mutants of a class A beta-lactamase.

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Prediction and experimental testing of Bacillus acidocaldarius thioredoxin stability1

Biochemical Journal ◽

10.1042/bj3390309 ◽

1999 ◽

Vol 339 (2) ◽

pp. 309-317 ◽

Cited By ~ 7

Author(s):

Emilia PEDONE ◽

Raffaele CANNIO ◽

Michele SAVIANO ◽

Mosè ROSSI ◽

Simonetta BARTOLUCCI

Keyword(s):

Protein Stability ◽

Molecular Dynamic ◽

Experimental Testing ◽

Ion Pairs ◽

Cd Spectroscopy ◽

Site Directed Mutagenesis ◽

Wild Type ◽

Type Protein ◽

Wild Type Protein ◽

Reference Protein

In order to investigate further the determinants of protein stability, four mutants of thioredoxin from Bacillus acidocaldarius were designed: K18G, R82E, K18G/R82E, and D102X, in which the last four amino acids were deleted. The mutants were constructed on the basis of molecular dynamic studies and the prediction of the structure of thioredoxin from B. acidocaldarius, performed by a comparative molecular modelling technique using Escherichia coli thioredoxin as the reference protein. The mutants obtained by PCR strategy were expressed in E. coli and then characterized. CD spectroscopy, spectrofluorimetry and thermodynamic comparative studies permitted comparison of the relative physicochemical behaviour of the four proteins with that of the wild-type protein. As predicted for the molecular dynamic analysis at 500 K in vacuo, the wild-type structure was more stable than that of the mutants; in fact the Tm of the four proteins showed a decrease of about 15 °C for the double and the truncated mutants, and a decrease of about 12 °C for the single mutants. A difference in the resistance of the proteins to denaturants such as guanidine HCl and urea was revealed; the wild-type protein always proved to be the most resistant. The results obtained show the importance of hydrogen bonds and ion pairs in determining protein stability and confirm that simulation methods are able to direct protein engineering in site-directed mutagenesis.

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Catalytic mechanism of active-site serine β-lactamases: role of the conserved hydroxy group of the Lys-Thr(Ser)-Gly triad

Biochemical Journal ◽

10.1042/bj3010485 ◽

1994 ◽

Vol 301 (2) ◽

pp. 485-494 ◽

Cited By ~ 35

Author(s):

A Dubus ◽

J M Wilkin ◽

X Raquet ◽

S Normark ◽

J M Frère

Keyword(s):

Hydroxy Group ◽

Catalytic Mechanism ◽

Site Directed Mutagenesis ◽

Peptidase Activity ◽

Beta Lactams ◽

Beta Lactamases ◽

Penicillin Binding Proteins ◽

Class A ◽

Class C

The role of the conserved hydroxy group of the Lys-Thr(Ser)-Gly [KT(S)G] triad has been studied for a class A and a class C beta-lactamase by site-directed mutagenesis. Surprisingly, the disappearance of this functional group had little impact on the penicillinase activity of both enzymes. The cephalosporinase activity was much more affected for the class A S235A (Ser235-->Ala) and the class C T316V (Thr315-->Val) mutants, but the class C T316A mutant was less impaired. Studies were extended to beta-lactams, where the carboxy group on C-3 of penicillins or C-4 of cephalosporins had been modified. The effects of the mutations were the same on these compounds as on the unmodified regular penicillins and cephalosporins. The results are compared with those obtained with a similar mutant (T299V) of the Streptomyces R61 DD-peptidase. With this enzyme the mutation also affected the interactions with penicillins and severely decreased the peptidase activity. The strict conservation of the hydroxy group on the second residue of the KT(S)G triad is thus much more easy to understand for the DD-peptidase and the penicillin-binding proteins than for beta-lactamases, especially those of class C.

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Effect of C-domain N-glycosylation and deletion on rat pancreaticα-amylase secretion and activity

Biochemical Journal ◽

10.1042/bj3620259 ◽

2002 ◽

Vol 362 (2) ◽

pp. 259-264 ◽

Cited By ~ 11

Author(s):

Yannick DOYON ◽

William HOME ◽

Philippe DAULL ◽

Denis LeBEL

Keyword(s):

Enzyme Activity ◽

Animal Cell ◽

Brefeldin A ◽

Enzymic Activity ◽

Site Directed Mutagenesis ◽

Amylase Secretion ◽

Wild Type ◽

Terminal Domain ◽

Relative Independence ◽

Asparagine Residue

Even though all animal α-amylases include glycosylation sequons (Asn-Xaa-Thr/Ser) in their sequences, amylases purified from natural sources are not quantitatively glycosylated. When wild-type rat pancreatic α-amylase, which contains two glycosylation sequons, was expressed in animal cell lines the protein displayed a very low rate of glycosylation (approx. 2%), even after Brefeldin A treatment to increase the contact with the glycosylation machinery. Site-directed mutagenesis of the first glycosylation sequon (Asn410 → Gln) resulted in 90% of the protein being glycosylated at the second glycosylation sequon (Asn459). Mutation of the second sequon completely inhibited glycosylation. In order to ascertain if the interference in the glycosylation of Asn459 that was eliminated by the Asn410 →Gln mutation could be due to the position of the asparagine residue in the Cys448-Cys460 disulphide bridge, these cysteine residues were mutated to serine residues. The resulting mutant was found to be 100% glycosylated. All mutants with mutations in the C-domain had specific activities identical to that of the wild-type enzyme, indicating that enzymic activity is independent of the structure and modification of the C-terminal domain. To further test the independence of the C-domain with respect to the two N-terminal domains of the protein, which harbour the catalytic site, the last seven of the ten β-strands that make up the β-sandwich configuration of the domain were deleted. The truncated protein was not secreted from cells and all enzyme activity was destroyed. These observations show that Asn459 is the only site that can be glycosylated in wild-type amylase, and confirm the relative independence of the C-terminal domain of α-amylase with respect to enzyme activity. In addition, they also establish that the C-terminal domain is absolutely essential for the correct post-translational folding of the enzyme that is responsible for its activity and allows for its secretion.

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