Unfolding of bacteriophage P22 tailspike protein: enhanced thermal stability of an N‐terminal fusion mutant

Carbonell, Xavier; Villaverde, Antonio

doi:10.1016/s0014-5793(98)00876-x

Cited by 8 publications

(3 citation statements)

References 21 publications

(34 reference statements)

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“…P22 TSP was also treated with trypsin in the presence of 2% SDS, migrated at 126 KDa size, which corresponds to 215 KDa size of the P22 TSP trimer in actual calculated molecular weight. Similar reports of migration characteristics of the trimeric protein of P22 in a 7.5% polyacrylamide gel has been published by X. Carbonell and A. Villaverde, indicating a 126±3 KDa migration in gel but an actual size of 215 KDa [57]. As depicted in Figure 3B, EEUTUH (the extended Ɛ34 TSP untreated and unheated) recorded the trimeric species migrating at blurry consistency at averagely 161 KDa.…”

Section: Partial Sensitivity Of Eɛ34 Tsp In 2% Sds To Trypsinsupporting

confidence: 86%

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Ɛ34 Phage Tailspike Protein is Resistant to Trypsin and Inhibits and Salmonella Biofilm Formation

Ayariga¹,

Gildea²,

Villafañe³

2021

Preprint

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Salmonella can cause acute and chronic infections in humans. Salmonella species are known to cause food poisoning and other diseases in developing countries. Their role in the pathogenesis of these diseases has received increased international attention. Despite numerous advances in sanitation, they still can infect humans and cause outbreaks in developed countries. For example, Salmonella causes about 1.2 million illnesses in the US each year with over 450 deaths. Additionally, Salmonella outbreaks cause significant losses to chicken producers globally. The Salmonella species is also prone to acquiring resistance to various classes of antibiotics. Hence, the need for a paradigm shift from antibiotics to bacteriophages to manage, control and treat bacterial infections. The ɛ34 phage belongs to Podoviruses and categorized into the P22-like phages. The P22-like phages include ɛ34, ES18, P22, ST104, and ST64T. In this work, we investigated the antibacterial property of ɛ34 phage tailspike protein against Salmonella newington (S. newington). We demonstrate here that, the phage’s tailspike protein enzymatic property as a LPS hydrolase synergizes with Vero Cell culture supernatant in killing S. newington. Using decellularized cartilage scaffold as an ex vivo tissue model, the ɛ34 TSP protected the scaffold from S. newington biofilm formation. Computational analysis of the ɛ34 TSP interaction with membrane proteins of S. newington demonstrated a higher probability (0.7318) of binding to ompA of S. newington, and when docked to ompA extracellular component, it produced a high free energy of -11.3kcal/mol. We also demonstrate the resistance/sensitivity of the tailspike to the digestive enzyme trypsin. The data obtained in this work indicates that the trypsin resistant tailspike protein of Ɛ34 phage can be formulated as a novel antibacterial agent against S. newington.

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Section: Partial Sensitivity Of Eɛ34 Tsp In 2% Sds To Trypsinsupporting

confidence: 86%

“…P22 TSP was also treated with trypsin as shown in eighth lane of same Figure 3B. A single band was observed at 126 KDa, which corresponds to 215 KDa size of the P22 TSP trimer in actual calculated molecular weight similar to reports by Carbonell and Villaverde [58].…”

Section: Partial Sensitivity Of Eɛ34 Tsp In 2% Sds To Trypsinsupporting

confidence: 79%

Ɛ34 Phage Tailspike Protein is Resistant to Trypsin and Inhibits and Salmonella Biofilm Formation

Ayariga¹,

Gildea²,

Villafañe³

2021

Preprint

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“…TSP is a homotrimeric protein that undergoes a complex folding pathway from which unfolded intermediates collapse as IBs under overproduction conditions [17,18]. In addition, TSP has been extensively used as a model for the analysis of molecular interactions between aggregated polypeptides [19] and of protein folding and unfolding pathways [20–24]. The arrest of recombinant protein synthesis in IB‐carrying cells results, as in the case of β‐galactosidase, in IB disintegration (Fig.…”

Section: Resultsmentioning

confidence: 99%

Protein aggregation as bacterial inclusion bodies is reversible

2001

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Inclusion bodies are refractile, intracellular protein aggregates usually observed in bacteria upon targeted gene overexpression. Since their occurrence has a major economical impact in protein production bio-processes, in vitro refolding strategies are under continuous exploration. In this work, we prove spontaneous in vivo release of both L L-galactosidase and P22 tailspike polypeptides from inclusion bodies resulting in their almost complete disintegration and in the concomitant appearance of soluble, properly folded native proteins with full biological activity. Since, in particular, the tailspike protein exhibits an unusually slow and complex folding pathway involving deep interdigitation of L L-sheet structures, its in vivo refolding indicates that bacterial inclusion body proteins are not collapsed into an irreversible unfolded state. Then, inclusion bodies can be observed as transient deposits of folding-prone polypeptides, resulting from an unbalanced equilibrium between in vivo protein precipitation and refolding that can be actively displaced by arresting protein synthesis. The observation that the formation of big inclusion bodies is reversible in vivo can be also relevant in the context of amyloid diseases, in which deposition of important amounts of aggregated protein initiates the pathogenic process. ß

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Connection between gene dosage and protein stability revealed by a high‐yield production of recombinant proteins in an E. coli LexA1(Ind⁻) background

Medina

Carbonell

Villaverde

2002

Biotech & Bioengineering

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Bacterial production of a plasmid-encoded bacteriophage P22 tailspike protein shows different yield and impact on cell viability in RecA+ LexA+, RecA- LexA+ and RecA+ LexA1(Ind-) backgrounds. In a LexA1(Ind-) context, we have observed lesser toxicity and higher productivity than in the wild-type strain, in which the bacterial growth was inhibited after induction of recombinant gene expression. Also, a negative effect of the incubation temperature on the growth of producing cells was also detected. By exploring the molecular basis of these inhibitory events, we found a connection between the dosage of the recombinant gene and the proteolytic stability of the encoded protein. Under both genetic and environmental conditions favoring higher plasmid copy number and consequently increasing the synthesis rate of the recombinant protein, enhanced protein degradation was observed in parallel with an important growth inhibition. Altogether, the obtained data suggest the existence of a critical concentration of recombinant protein over which cell proteolysis is stimulated at rates not compatible with optimal physiological conditions for bacterial growth.

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Unfolding of bacteriophage P22 tailspike protein: enhanced thermal stability of an N‐terminal fusion mutant

Cited by 8 publications

References 21 publications

Ɛ34 Phage Tailspike Protein is Resistant to Trypsin and Inhibits and Salmonella Biofilm Formation

Ɛ34 Phage Tailspike Protein is Resistant to Trypsin and Inhibits and Salmonella Biofilm Formation

Protein aggregation as bacterial inclusion bodies is reversible

Connection between gene dosage and protein stability revealed by a high‐yield production of recombinant proteins in an E. coli LexA1(Ind⁻) background

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Unfolding of bacteriophage P22 tailspike protein: enhanced thermal stability of an N‐terminal fusion mutant

Cited by 8 publications

References 21 publications

Ɛ34 Phage Tailspike Protein is Resistant to Trypsin and Inhibits and Salmonella Biofilm Formation

Ɛ34 Phage Tailspike Protein is Resistant to Trypsin and Inhibits and Salmonella Biofilm Formation

Protein aggregation as bacterial inclusion bodies is reversible

Connection between gene dosage and protein stability revealed by a high‐yield production of recombinant proteins in an E. coli LexA1(Ind−) background

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Connection between gene dosage and protein stability revealed by a high‐yield production of recombinant proteins in an E. coli LexA1(Ind⁻) background