Secreted Antibody/Granzyme B Fusion Protein Stimulates Selective Killing of HER2-overexpressing Tumor Cells

Abstract: HER2/ErbB2, an epidermal growth factor receptor-related tyrosine kinase, is overexpressed on the surface of a variety of tumors of epithelial origin, such as breast tumors, ovarian carcinomas, and gastric tumors, and therefore constitutes an ideal therapeutic target (1-3). Among the many advances in the development of HER2-targeted cancer therapy over the past decade (4 -7), antibody-based strategies (e.g. herceptin (trastuzumab) (8 -10), intracellular antibody (11, 12), and fusion proteins for targeted delive… Show more

“…Three PEA II domain variants, C-terminally truncated PEA II domain (PEA253-358 aa), both C-terminally and N-terminally truncated PEA II domain (PEA275-358 aa), and one short sequence containing only a furin cleavage site (PEA275-280 aa) were successfully fused to a single-chain antibody against HER2(e23sFv) 13,14 and constitutively active granzyme B. The recombinant genes were subcloned downstream and in frame with DNA encoding a signal sequence (MKHLWFFLLLVAAPRWVLS) in the expression vector pCMV.…”

“…A signal sequence was also introduced in the constructs to ensure that all the recombinant proteins were secreted. 13 We monitored translocation activities indirectly by measuring cytotoxicity of ImmunoGrB fusion protein as well as directly by immunofluorescence.…”

“…8,9 Although earlier studies used PEA fragment from amino acids 253-412 or 253-364 for protein translocation, these data suggested that amino acids 253-358 is sufficient for PEA translocation. [10][11][12][13] In order to determine the minimum domain length required for translocation, a set of deletions in the PEA translocation domain were introduced into the previously constructed ImmunoGrB, 13 which is composed of a single-strand antibody against HER2, translocation domain from PEA, and active granzyme B. A signal sequence was also introduced in the constructs to ensure that all the recombinant proteins were secreted.…”

HER2-targeting recombinant protein with truncated Pseudomonas Exotoxin: A translocation domain efficiently kills breast cancer cells

“…Three PEA II domain variants, C-terminally truncated PEA II domain (PEA253-358 aa), both C-terminally and N-terminally truncated PEA II domain (PEA275-358 aa), and one short sequence containing only a furin cleavage site (PEA275-280 aa) were successfully fused to a single-chain antibody against HER2(e23sFv) 13,14 and constitutively active granzyme B. The recombinant genes were subcloned downstream and in frame with DNA encoding a signal sequence (MKHLWFFLLLVAAPRWVLS) in the expression vector pCMV.…”

“…A signal sequence was also introduced in the constructs to ensure that all the recombinant proteins were secreted. 13 We monitored translocation activities indirectly by measuring cytotoxicity of ImmunoGrB fusion protein as well as directly by immunofluorescence.…”

“…8,9 Although earlier studies used PEA fragment from amino acids 253-412 or 253-364 for protein translocation, these data suggested that amino acids 253-358 is sufficient for PEA translocation. [10][11][12][13] In order to determine the minimum domain length required for translocation, a set of deletions in the PEA translocation domain were introduced into the previously constructed ImmunoGrB, 13 which is composed of a single-strand antibody against HER2, translocation domain from PEA, and active granzyme B. A signal sequence was also introduced in the constructs to ensure that all the recombinant proteins were secreted.…”

HER2-targeting recombinant protein with truncated Pseudomonas Exotoxin: A translocation domain efficiently kills breast cancer cells

“…There the translocation domain of a bacterial toxin was included in the molecule to achieve cytoplasmic delivery of an active GrB fragment in target cells. 35 In the presence of chloroquine, GrB-5 and GrB-T were able to specifically kill target cells with IC 50 values in the picomolar to nanomolar range, whereas nontarget cells were not affected at considerably higher concentrations. These cytotoxic activities of the chimeric GrB derivatives are comparable to those of Pseudomonas exotoxin A fusion proteins which employ the same cell targeting domains.…”

“…In another approach, the problem to produce a functional tumor-specific GrB fusion protein was solved by coincubating tumor cells with engineered T cells releasing such a molecule. 35 We have followed a different strategy expressing the ErbB2-specific GrB-5 and EGFR-specific GrB-T molecules as secreted proteins in the yeast P. pastoris, thereby bypassing the need for refolding or in vitro activation, and resulting in large amounts of active recombinant proteins after a single purification step. Attachment of the C-terminal antibody and growth factor domains did not affect enzymatic activity of GrB.…”

Targeted induction of apoptosis by chimeric granzyme B fusion proteins carrying antibody and growth factor domains for cell recognition

Fusion Proteins with Toxic Activity