Validation of a mutant of the pore-forming toxin sticholysin-I for the construction of proteinase-activated immunotoxins

The use of pore-forming toxins from sea anemones (actinoporins) in the construction of immunotoxins (ITs) against tumour cells is an alternative for cancer therapy. However, the main disadvantage of actinoporin-based ITs obtained so far has been the poor cellular specificity associated with the toxi...

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Published in:Protein engineering, design and selection Vol. 24; no. 6; pp. 485 - 493
Main Authors: Pentón, David, Pérez-Barzaga, Victor, Díaz, Iscel, Reytor, Mey L., Campos, Javier, Fando, Rafael, Calvo, Loany, Cilli, Eduardo M., Morera, Vivian, Castellanos-Serra, Lila R., Pazos, Fabiola, Lanio, María E., Álvarez, Carlos, Pons, Tirso, Tejuca, Mayra
Format: Journal Article
Language:English
Published: England Oxford University Press 01-06-2011
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Abstract The use of pore-forming toxins from sea anemones (actinoporins) in the construction of immunotoxins (ITs) against tumour cells is an alternative for cancer therapy. However, the main disadvantage of actinoporin-based ITs obtained so far has been the poor cellular specificity associated with the toxin's ability to bind and exert its activity in almost any cell membrane. Our final goal is the construction of tumour proteinase-activated ITs using a cysteine mutant at the membrane binding region of sticholysin-I (StI), a cytolysin isolated from the sea anemone Stichodactyla helianthus. The mutant and the ligand moiety would be linked by proteinase-sensitive peptides through the StI cysteine residue blocking the toxin binding region and hence the IT non-specific killing activity. To accomplish this objective the first step was to obtain the mutant StI W111C, and to evaluate the impact of mutating tryptophan 111 by cysteine on the toxin pore-forming capacity. After proteolysis of the cleavage sequence, a short peptide would remain attached to the toxin. The next step was to evaluate whether this mutant is able to form pores even with a residual peptide linked to cysteine 111. In this work we demonstrated that (i) StI W111C shows pore-forming capacity in a nanomolar range, although it is 8-fold less active than the wild-type recombinant StI, corroborating the previously reported importance of residue 111 for the binding of StI to membranes, and (ii) the mutant is able to form pores even with a residual seven-residue peptide linked to cysteine 111. In addition, it was demonstrated that binding of a large molecule to cysteine 111 renders an inactive toxin that is no longer able to bind to the membrane. These results validate the mutant StI W111C for its use in the construction of tumour proteinase-activated ITs.
AbstractList The use of pore-forming toxins from sea anemones (actinoporins) in the construction of immunotoxins (ITs) against tumour cells is an alternative for cancer therapy. However, the main disadvantage of actinoporin-based ITs obtained so far has been the poor cellular specificity associated with the toxin's ability to bind and exert its activity in almost any cell membrane. Our final goal is the construction of tumour proteinase-activated ITs using a cysteine mutant at the membrane binding region of sticholysin-I (StI), a cytolysin isolated from the sea anemone Stichodactyla helianthus. The mutant and the ligand moiety would be linked by proteinase-sensitive peptides through the StI cysteine residue blocking the toxin binding region and hence the IT non-specific killing activity. To accomplish this objective the first step was to obtain the mutant StI W111C, and to evaluate the impact of mutating tryptophan 111 by cysteine on the toxin pore-forming capacity. After proteolysis of the cleavage sequence, a short peptide would remain attached to the toxin. The next step was to evaluate whether this mutant is able to form pores even with a residual peptide linked to cysteine 111. In this work we demonstrated that (i) StI W111C shows pore-forming capacity in a nanomolar range, although it is 8-fold less active than the wild-type recombinant StI, corroborating the previously reported importance of residue 111 for the binding of StI to membranes, and (ii) the mutant is able to form pores even with a residual seven-residue peptide linked to cysteine 111. In addition, it was demonstrated that binding of a large molecule to cysteine 111 renders an inactive toxin that is no longer able to bind to the membrane. These results validate the mutant StI W111C for its use in the construction of tumour proteinase-activated ITs.
Author Díaz, Iscel
Reytor, Mey L.
Castellanos-Serra, Lila R.
Pentón, David
Lanio, María E.
Fando, Rafael
Calvo, Loany
Morera, Vivian
Cilli, Eduardo M.
Campos, Javier
Álvarez, Carlos
Pazos, Fabiola
Pons, Tirso
Tejuca, Mayra
Pérez-Barzaga, Victor
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Keywords immunotoxin
actinoporin
sea anemone cytolysin
sticholysins
pore-forming toxin
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Snippet The use of pore-forming toxins from sea anemones (actinoporins) in the construction of immunotoxins (ITs) against tumour cells is an alternative for cancer...
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SubjectTerms Animals
Cell Membrane - chemistry
Cell Membrane - metabolism
Chromatography, Gel
Chromatography, Ion Exchange
Dimerization
Immunotoxins - chemistry
Immunotoxins - genetics
Immunotoxins - isolation & purification
Immunotoxins - metabolism
Marine
Models, Molecular
Mutation
Organic Chemicals - chemistry
Organic Chemicals - isolation & purification
Organic Chemicals - metabolism
Perforin
Pore Forming Cytotoxic Proteins - chemistry
Pore Forming Cytotoxic Proteins - genetics
Pore Forming Cytotoxic Proteins - isolation & purification
Pore Forming Cytotoxic Proteins - metabolism
Protein Binding
Reproducibility of Results
Sea Anemones
Stichodactyla helianthus
Title Validation of a mutant of the pore-forming toxin sticholysin-I for the construction of proteinase-activated immunotoxins
URI https://www.ncbi.nlm.nih.gov/pubmed/21296830
https://search.proquest.com/docview/907174998
Volume 24
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