Combination of antibody targeting and PTD-mediated intracellular toxin delivery for colorectal cancer therapy

Shin, Meong Cheol; Zhang, Jian; Min, Kyung Up; Lee, Kyuri; Moon, Cheol; Balthasar, Joseph P.; Yang, Victor C.

doi:10.1016/j.jconrel.2014.08.030

Cited by 50 publications

(38 citation statements)

References 47 publications

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“…This approach was further examined in a LS174T-xenograft model, which resulted in increased intratumoral accumulation and inhibition of tumor growth (46%). This finding demonstrates the potential usefulness of a CPP for enhancing antibody-promoted active targeting [56].…”

Section: Antibody-and/or Ligand-combined Cpp Deliverymentioning

confidence: 52%

“…For example, the TAT-conjugated plant-derived protein toxin geolin binds to a conjugate of heparin (Hep) and a murine anticarcinoembryonic antigen monoclonal antibody (anti-CEA mAb, T84.66) through an electrostatic interaction between TAT and Hep [56]. This complex, when attached to CEA-overexpressing LS174T colorectal cancer cells, slowly released TAT-geolin, which was then internalized by the cancer cells.…”

Section: Antibody-and/or Ligand-combined Cpp Deliverymentioning

confidence: 99%

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Cell-penetrating peptides: strategies for anticancer treatment

Raucher

Ryu

2015

Trends in Molecular Medicine

200

159

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Section: Antibody-and/or Ligand-combined Cpp Deliverymentioning

confidence: 52%

Section: Antibody-and/or Ligand-combined Cpp Deliverymentioning

confidence: 99%

Cell-penetrating peptides: strategies for anticancer treatment

Raucher

Ryu

2015

Trends in Molecular Medicine

200

159

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“…As a fusion partner, TRX is a small 12-kDa redox protein that can be overexpressed to a high level in E coli (accumulation of up to 40% of the cellular proteins) in a soluble form [28] . The utility of TRX as a fusion partner for soluble expression of gelonin fusion proteins has already been reported in our previous publications [24,29] . Herein, we have clearly demonstrated the plausibility of this strategy, as the N-terminal thioredoxin-6×His tagged-gelonin-F3 peptide chimera (F3-Gel) was successfully produced in large quantities as a soluble protein in E coli.…”

Section: Discussionmentioning

confidence: 78%

Molecular tumor targeting of gelonin by fusion with F3 peptide

2017

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Therapeutically potent macromolecular drugs have shown great promise for overcoming the limitations of small-molecule anti-cancer drugs. But tumor cell-selective intracellular delivery of the macromolecules remains a major hurdle for their successful clinical application. To overcome this challenge, we engineered a novel genetic fusion protein (F3-Gel) that composed of F3 peptide, a tumorhoming peptide, and gelonin, a plant-derived ribosome-inactivating protein (RIP), and then evaluated its anti-cancer activity in vitro and in vivo. The F3-Gel-encoding gene was synthesized by genetic recombination, and F3-Gel was successfully expressed in E coli. The anti-cancer activity of the produced F3-Gel was evaluated by various in vitro assays, which revealed that F3-Gel maintained equipotent protein synthesis inhibition activity (IC 50 =11 pmol/L) as unmodified gelonin (IC 50 =10 pmol/L). Furthermore, F3-Gel displayed enhanced cellular uptake into cancer cells (U87 MG, HeLa, LnCaP and 9L) than noncancerous cells (293 HEK and SVGp12). Compared with gelonin, F3-Gel exerted significantly higher cytotoxicity against these cancer cells. F3-Gel displayed significantly greater inhibition of protein translation in U87 MG cells: F3-Gel (0.5 μmol/L) was able to reduce the protein level to less than 50%, while gelonin (1 μmol/L) did not affect the intracellular protein level. In a U87 MG xenograft tumor-bearing mouse model, F3-Gel was accumulated in the tumor site at much higher levels and maintained for a prolonged time compared with gelonin. Administration of F3-Gel (0.5, 0.75 mol/kg, iv) caused 36% and 66%, respectively, inhibition of tumor growth in U87 MG xenograft mice, suggesting that it is a promising candidate drug for cancer treatment. Furthermore, this study demonstrates that fusion of F3 peptide to a potent macromolecule could provides an effective method for targeting tumors and eventually could improve their druggability.

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“…To this regards, in this research, we explored the feasibility of applying the PTD-modified ATTEMPTS for effective yet safe administration of TAT-Gel, by utilizing a heparin functionalized anti-carcinoembryonic antigen (CEA) mAb, T84.66-Hep that showed feasible tumor targeting of TAT-Gel in our previous studies (24), as the targeting component and protamine as the trigger release agent. After in vitro characterization of the CEA binding specificity and cell internalization of T84.66-Hep, we prepared an antibody/toxin complex by mixing the T84.66-Hep and TAT-Gel.…”

Section: Introductionmentioning

confidence: 99%

PTD-Modified ATTEMPTS for Enhanced Toxin-based Cancer Therapy: An In Vivo Proof-of-Concept Study

et al. 2015

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Purpose To investigate the feasibility of applying PTD-modified ATTEMPTS (Antibody Targeted Triggered Electrically Modified Prodrug-Type Strategy) for enhanced toxin therapy for the treatment of cancer. Methods A heparin-functionalized murine anti-CEA monoclonal antibody (mAb), T84.66-heparin (T84.66-Hep), was chemically synthesized and characterized for specific binding to CEA overexpressed cells. The T84.66-Hep was then applied to the PTD-modified ATTEMPTS approach and the crucial features of the drug delivery system (DDS), ‘antibody targeting’ and ‘heparin/protamine-based prodrug’, were evaluated in vitro to examine whether it could selective delivery a PTD-modified toxin, recombinant TAT-gelonin chimera (TAT-Gel), to CEA high expression cancer cells (LS174T). Furthermore, the feasibility of the drug delivery system (DDS) was assessed in vivo by biodistribution and efficacy studies using LS174T s.c. xenograft tumor bearing mice. Results T84.66-Hep displayed specific binding, but limited internalization (35% after 48 h incubation) to CEA high expression LS174T cells over low expression HCT116 cells. When mixed together with TAT-Gel, the T84.66-Hep formed a strong yet reversible complex. This complex formation provided an effective means of active tumor targeting of TAT-Gel, by 1) directing the TAT-Gel to CEA overexpressed tumor cells and 2) preventing nonspecific cell transduction to non-targeted normal cells. The cell transduction of TAT-Gel could, however, be efficiently reversed by addition of protamine. Feasibility of in vivo tumor targeting and “protamine-induced release” of TAT-Gel from the T84.66-Hep counterpart was confirmed by biodistribution and preliminary efficacy studies. Conclusions This study successfully demonstrated in vitro and in vivo the applicability of PTD-modified ATTEMPTS for toxin-based cancer therapy.

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Combination of antibody targeting and PTD-mediated intracellular toxin delivery for colorectal cancer therapy

Cited by 50 publications

References 47 publications

Cell-penetrating peptides: strategies for anticancer treatment

Cell-penetrating peptides: strategies for anticancer treatment

Molecular tumor targeting of gelonin by fusion with F3 peptide

PTD-Modified ATTEMPTS for Enhanced Toxin-based Cancer Therapy: An In Vivo Proof-of-Concept Study

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