The potent mitogen <i>Pasteurella multocida</i> toxin is highly resistant to proteolysis but becomes susceptible at lysosomal pH

Smyth, Martin G.; Pickersgill, Richard W.; Lax, Alistair J.

doi:10.1016/0014-5793(95)00077-m

Cited by 19 publications

(25 citation statements)

References 31 publications

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“…PMT has previously been shown to be highly resistant to most proteases at neutral pH (46). One protease, Asp-N, was found to cleave PMT at pH 7, producing three fragments of ca.…”

Section: Resultsmentioning

confidence: 99%

“…One protease, Asp-N, was found to cleave PMT at pH 7, producing three fragments of ca. 90, 87, and 55 kDa (46). Amino-terminal sequencing of these fragments showed that the toxin was cleaved between residues 473 and 474, and between 509 and 510.…”

Section: Resultsmentioning

confidence: 99%

“…Its action is also inhibited by neutralizing antibody or methylamine added early but not late after toxin. PMT undergoes a conformational change at low pH, which affects its protease sensitivity and circular dichroism spectra (46,47). This suggests that PMT may be trafficked and perhaps processed through a low-pH compartment.…”

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confidence: 99%

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Localization of Functional Domains of the Mitogenic Toxin of Pasteurella multocida

2001

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The locations of the catalytic and receptor-binding domains of the Pasteurella multocida toxin (PMT) were investigated. N-and C-terminal fragments of PMT were cloned and expressed as fusion proteins with affinity tags. Purified fusion proteins were assessed in suitable assays for catalytic activity and cell-binding ability. A C-terminal fragment (amino acids 681 to 1285) was catalytically active. When microinjected into quiescent Swiss 3T3 cells, it induced changes in cell morphology typical of toxin-treated cells and stimulated DNA synthesis. An N-terminal fragment with a His tag at the C terminus (amino acids 1 to 506) competed with full-length toxin for binding to surface receptors and therefore contains the cell-binding domain. The inactive mutant containing a mutation near the C terminus (C1165S) also bound to cells in this assay. Polyclonal antibodies raised to the N-terminal PMT region bound efficiently to full-length native toxin, suggesting that the N terminus is surface located. Antibodies to the C terminus of PMT were microinjected into cells and inhibited the activity of toxin added subsequently to the medium, confirming that the C terminus contains the active site. Analysis of the PMT sequence predicted a putative transmembrane domain with predicted hydrophobic and amphipathic helices near the N terminus over the region of homology to the cytotoxic necrotizing factors. The C-terminal end of PMT was predicted to be a mixed ␣/␤ domain, a structure commonly found in catalytic domains. Homology to proteins of known structure and threading calculations supported these assignments.

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“…PMT has previously been shown to be highly resistant to most proteases at neutral pH (46). One protease, Asp-N, was found to cleave PMT at pH 7, producing three fragments of ca.…”

Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

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Localization of Functional Domains of the Mitogenic Toxin of Pasteurella multocida

2001

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“…The toxin is passively released upon bacterial lysis and is believed to be actively taken up by host cells via receptor -mediated endocytosis by binding to a ganglioside cell surface receptor (Pettit et al 1993 ). The N -terminal receptor -binding domain is then proteolytically cleaved under low pH conditions (Smyth et al 1995 ), exposing the translocation domain, which allows uptake into the cytoplasm . Here the catalytic C -terminal portion of the protein activates two heterotrimeric G proteins, G α q and G α 12/13 , which in turn affect a number of host signal transduction pathways ).…”

Section: Pmtmentioning

confidence: 99%

Pasteurella

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et al. 2010

Pathogenesis of Bacterial Infections in Animals

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“…The translocation depends on a putative translocation T-domain, consisting of two predicted hydrophobic helices (residues 402-423 and 437-457) linked by a peptide loop (residues 424-436). It is proposed that acidification induces a structural change in the toxin, which was previously observed utilising circular dichroism and measuring susceptibility to proteases (Smyth et al 1995(Smyth et al , 1999. This structural change exposes the T-domain, allowing it to insert into the vesicular membrane.…”

Section: Uptake Into Eukaryotic Cellsmentioning

confidence: 96%