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Humanin

HN, S14G-Humanin

Quick Stats
Studies 491
Trials 100
Overview Studies Clinical Trials
Score 3
2015 pubmed 40 citations

The effects of humanin and its analogues on male germ cell apoptosis induced by chemotherapeutic drugs.

Jia. Yue Y; Ohanyan. Aikoui A; Lue. Yan-He YH; Swerdloff. Ronald S RS; Liu. Peter Y PY; Cohen. Pinchas P; Wang. Christina C

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Key Findings

  • Humanin and its analogues reduced chemotherapy‑induced apoptosis of male germ cells in mice
  • The protective effect operates mainly via a membrane receptor and STAT3 activation, with little role for BAX or IGFBP‑3 binding
  • An antagonist analogue blocked protection, confirming the specificity of humanin’s action

Practical Outcomes

  • Humanin shows promise as a fertility‑protective agent during chemo, but there are no human studies, dosing guidelines, or approved formulations yet. Biohackers should wait for clinical data before trying it, and focus on established fertility‑preserving strategies for now.

Summary

Humanin, a tiny protein made by our cells, was shown to protect male sperm‑producing cells from the damage caused by chemotherapy drugs in mouse studies. Several modified versions of humanin worked similarly, acting mainly through a cell‑surface receptor and a signaling pathway called STAT3. This suggests humanin could someday help preserve male fertility during cancer treatment, but we still need human trials and dosage info before anyone can safely use it themselves.

Abstract

Human (HN) prevents stress-induced apoptosis in many cells/tissues. In this study we showed that HN ameliorated chemotherapy [cyclophosphamide (CP) and Doxorubicin (DOX)]-induced male germ cell apoptosis both ex vivo in seminiferous tubule cultures and in vivo in the testis. HN acts by several putative mechanisms via binding to: an IL-12 like trimeric membrane receptor; BAX; or insulin-like growth factor binding protein-3 (IGFBP-3, a proapoptotic factor). To understand the mechanisms of HN on male germ cell apoptosis, we studied five HN analogues including: HNG (HN-S14G, a potent agonist), HNG-F6A (no binding to IGFBP-3), HN-S7A (no self-dimerization), HN-C8P (no binding to BAX), and HN-L12A (a HN antagonist) on CP-induced male germ cell apoptosis in mice. CP-induced germ cell apoptosis was inhibited by HN, HNG, HNG-F6A, HN-S7A, and HN-C8P (less effective); but not by HN-L12A. HN-L12A, but not HN-S7A or HN-C8P, blocked the protective effect of HN against CP-induced male germ cell apoptosis. HN, HN-S7A, and HN-C8P restored CP-suppressed STAT3 phosphorylation. These results suggest that HN: (1) decreases DOX (ex vivo) and CP (in vivo) induced male germ cell apoptosis; (2) action is mediated by the membrane receptor/STAT3 with minor contribution by BAX-binding pathway; (3) self-dimerization or binding to IGFBP-3 may not be involved in HN's effect in testis. HN is an important molecule in the regulation of germ cell homeostasis after injury and agonistic analogues may be developed for treating male infertility or protection against chemotherapy side effects.

Study Information

Provider

pubmed

Year

2015

Date

2015-02-10T00:00:00.000Z

DOI

10.1007/s10495-015-1105-5

Citations

40

References

53