The penetratin sequence in the anticancer PNC-28 peptide causes tumor cell necrosis rather than apoptosis of human pancreatic cancer cells.
Bowne. Wilbur B WB; Sookraj. Kelley A KA; Vishnevetsky. Michael M; Adler. Victor V; Sarafraz-Yazdi. Ehsan E; Lou. Sunming S; Koenke. Jesco J; Shteyler. Vadim V; Ikram. Kamran K; Harding. Michael M; Bluth. Martin H MH; Ng. Mou M; Brandt-Rauf. Paul W PW; Hannan. Raqibul R; Bradu. Stephan S; Zenilman. Michael E ME; Michl. Josef J; Pincus. Matthew R MR
Key Findings
- PNC‑28 (p53 aa17‑26 + penetratin) causes rapid necrotic death of human pancreatic cancer cells, measured by LDH release and membrane pore formation.
- The penetratin sequence is essential for this necrotic mechanism; a similar peptide without penetratin (or expressed from a plasmid) leads to apoptosis instead.
- Normal, non‑cancerous pancreatic cells were not killed by PNC‑28, indicating some tumor selectivity in vitro.
Practical Outcomes
- For DIY health enthusiasts, the study suggests that attaching penetratin to short p53‑derived peptides can dramatically change how they kill cancer cells, but the work is limited to cell cultures and provides no dosage, safety, or delivery guidance for humans. Until animal or clinical data are available, it remains a mechanistic insight rather than a ready‑to‑use protocol.
Summary
A lab study found that adding a cell‑penetrating tag called penetratin to a short p53‑derived peptide (PNC‑28) makes it kill pancreatic cancer cells by bursting their membranes (necrosis) instead of the usual programmed cell death (apoptosis). Without the penetratin tag, the same peptide only triggers apoptosis. The effect was seen in cancer cells but not in normal pancreatic cells.
Abstract
PNC-27 and PNC-28 are p53-derived peptides from the human double minute (hdm-2) binding domain attached to penetratin. These peptides induce tumor cell necrosis of cancer cells, but not normal cells. The anticancer activity and mechanism of PNC-28 (p53 aa17-26-penetratin) was specifically studied against human pancreatic cancer. MiaPaCa-2 cells were treated with PNC-28. Necrosis was determined by measuring lactate dehydrogenase (LDH) and apoptosis as assayed for measuring elevation of proapoptotic proteins. PNC-29, an unrelated peptide, and hdm-2-binding domain p53 aa12-26 without penetratin (PNC-26) were used as controls. Since there is evidence that penetratin is required for tumor cell necrosis, we tested "naked" p53 peptide without penetratin by transfecting a plasmid that encodes p53 aa17-26 segment of PNC-28 into MiaPaCa-2 and an untransformed rat pancreatic acinar cell line, BMRPA1. Time-lapse electron microscopy was employed to further elucidate anticancer mechanism. Treatment with PNC-28 does not result in the elevation of proapoptotic proteins found in p53-induced apoptosis, but elicits rapid release of LDH, indicative of tumor cell necrosis. Accordingly, we observed membrane pore formation and dose-dependent killing. In direct contrast, transfected MiaPaCa-2 cells underwent apoptosis, and not necrosis, as evidenced by expression of high levels of caspases-3 and 7 and annexin V with background levels of LDH. These results suggest that PNC-28 may be effective in treating human pancreatic cancer. The penetratin sequence appears to be responsible for the fundamental change in the mechanism of action, inducing rapid necrosis initiated by membrane pore formation. Cancer cell death by apoptosis was observed in the absence of penetratin.
Study Information
pubmed
2008
2008-10-18T00:00:00.000Z
10.1245/s10434-008-0147-0
16
16