. 2015 Aug;21(8):825-31.

doi: 10.1089/ten.TEC.2014.0500. Epub 2015 Apr 15.

Cryopreservation of the Hair Follicle Maintains Pluripotency of Nestin-Expressing Hair Follicle-Associated Pluripotent Stem Cells

Affiliations

¹ 1 Department of Dermatology, Kitasato University School of Medicine , Sagamihara, Japan .
² 2 Department of Physiology, Kitasato University School of Medicine , Sagamihara, Japan .
³ 3 AntiCancer, Inc. , San Diego, California.
⁴ 4 Department of Surgery, University of California San Diego , La Jolla, California.

PMID: 25743086
PMCID: PMC4523096
DOI: 10.1089/ten.TEC.2014.0500

Cryopreservation of the Hair Follicle Maintains Pluripotency of Nestin-Expressing Hair Follicle-Associated Pluripotent Stem Cells

Satoshi Kajiura et al. Tissue Eng Part C Methods. 2015 Aug.

. 2015 Aug;21(8):825-31.

doi: 10.1089/ten.TEC.2014.0500. Epub 2015 Apr 15.

Authors

Affiliations

¹ 1 Department of Dermatology, Kitasato University School of Medicine , Sagamihara, Japan .
² 2 Department of Physiology, Kitasato University School of Medicine , Sagamihara, Japan .
³ 3 AntiCancer, Inc. , San Diego, California.
⁴ 4 Department of Surgery, University of California San Diego , La Jolla, California.

PMID: 25743086
PMCID: PMC4523096
DOI: 10.1089/ten.TEC.2014.0500

Abstract

Hair follicles contain nestin-expressing pluripotent stem cells, the origin of which is above the bulge area, below the sebaceous gland. We have termed these cells hair follicle-associated pluripotent (HAP) stem cells. In the present study, we established efficient cryopreservation methods of the hair follicle that maintained the pluripotency of HAP stem cells. We cryopreserved the whole hair follicle from green fluorescent protein transgenic mice by slow-rate cooling in TC-Protector medium and storage in liquid nitrogen. After thawing, the upper part of the hair follicle was isolated and cultured in Dulbecco's Modified Eagle's Medium (DMEM) with fetal bovine serum (FBS). After 4 weeks of culture, cells from the upper part of the hair follicle grew out. The growing cells were transferred to DMEM/F12 without FBS. After 1 week of culture, the growing cells formed hair spheres, each containing ∼1×10(2) HAP stem cells. The hair spheres contained cells that differentiated to neurons, glial cells, and other cell types. The thawed and cultured upper part of the hair follicle produced almost as many pluripotent hair spheres as fresh follicles. The hair spheres derived from slow-cooling cryopreserved hair follicles were as pluripotent as hair spheres from fresh hair follicles. In contrast, rapid-cooling (vitrification) cryopreservation poorly preserved the pluripotency of the hair follicle stem cells. Stem cell marker genes (nestin, Sox2, and SSEA-1) were as highly expressed in slow-rate cooled cryopreserved follicles, after thawing, as in fresh follicles. However, in the vitrification cryopreserved follicles, the expression of the stem cell marker genes was greatly reduced. Direct cryopreservation of hair spheres by either the rapid-cooling, or slow-cooling method, resulted in loss of pluripotency. These results suggest that the slow-rate cooling cryopreservation of the whole hair follicle is effective to store HAP stem cells. Stored HAP stem cells would be very useful in personalized regenerative medicine, enabling any individual to maintain a bank of pluripotent stem cells for future clinical use.

PubMed Disclaimer

Figures

<b>FIG. 1.</b> — **FIG. 1.**
**(A)** Schema of slow-rate cooling and rapid-cooling (vitrification) methods of cryopreserving hair follicles and hair spheres. **(B)** Schema for dividing the hair follicle into upper, middle, and lower parts.

<b>FIG. 2.</b> — **FIG. 2.**
**(A)** Images demonstrating the recovery of sphere formation after cryopreservation by slow-rate cooling or rapid-cooling vitrification compared to fresh follicles. **(B)** Comparison of the attachment rate and growing cell number from fresh and cryopreserved hair follicles using slow-rate cooling or rapid-cooling vitrification after thawing and 4 weeks of culture in Dulbecco's Modified Eagle's Medium (DMEM) with 10% fetal bovine serum (FBS). Results are mean±standard deviation (SD) for three independent experiments (three independent mice for each method of cryopreservation and nonfrozen control). **(C)** Comparison of sphere number, produced from fresh follicles and follicles cryopreserved by slow-rate cooling or rapid-cooling vitrification, per upper part of the hair follicle. Results are mean±SD for three independent experiments (three samples each).

<b>FIG. 3.</b> — **FIG. 3.**
**(A)** Images demonstrating the recovery of differentiation potential after cryopreservation by slow-rate cooling or rapid-cooling vitrification compared to fresh follicles. *Red* color is for specific antibody staining and *blue* color is for nuclear staining. **(B)** Comparison of pluripotency of fresh hair follicles and hair follicles cryopreserved by slow-rate cooling or rapid-cooling vitrification after a one-week culture of hair spheres in DMEM with 10% FBS. Results are mean±SD for three independent experiments (three independent mice for each method of cryopreservation and nonfrozen control).

<b>FIG. 4.</b> — **FIG. 4.**
**(A)** Comparison of the mRNA levels of stem cell marker genes (nestin, Sox2, SSEA-1) were examined using real-time polymerase chain reaction (RT-PCR) analysis. Results are mean±SD for three samples each. The mRNA levels of stem cell marker genes were maintained in the slow-rate cooling method but significantly reduced in the rapid-cooling vitrification method. **(B)** Western-blot analysis was performed to detect the expression of SSEA-1. The protein level of SSEA-1 was maintained in the slow-rate cooling method but reduced in the rapid-cooling vitrification method.

See this image and copyright information in PMC

Cited by

Early-age-dependent selective decrease of differentiation potential of hair-follicle-associated pluripotent (HAP) stem cells to beating cardiac-muscle cells.
Yamazaki A, Hamada Y, Arakawa N, Yashiro M, Mii S, Aki R, Kawahara K, Hoffman RM, Amoh Y. Yamazaki A, et al. Cell Cycle. 2016 Oct;15(19):2619-2625. doi: 10.1080/15384101.2016.1208870. Epub 2016 Jul 18. Cell Cycle. 2016. PMID: 27428074 Free PMC article.
Implanted hair-follicle-associated pluripotent (HAP) stem cells encapsulated in polyvinylidene fluoride membrane cylinders promote effective recovery of peripheral nerve injury.
Yamazaki A, Obara K, Tohgi N, Shirai K, Mii S, Hamada Y, Arakawa N, Aki R, Hoffman RM, Amoh Y. Yamazaki A, et al. Cell Cycle. 2017 Oct 18;16(20):1927-1932. doi: 10.1080/15384101.2017.1363941. Epub 2017 Sep 8. Cell Cycle. 2017. PMID: 28886268 Free PMC article.
From hair to heart: nestin-expressing hair-follicle-associated pluripotent (HAP) stem cells differentiate to beating cardiac muscle cells.
Yashiro M, Mii S, Aki R, Hamada Y, Arakawa N, Kawahara K, Hoffman RM, Amoh Y. Yashiro M, et al. Cell Cycle. 2015;14(14):2362-6. doi: 10.1080/15384101.2015.1042633. Epub 2015 May 13. Cell Cycle. 2015. PMID: 25970547 Free PMC article.
Hair follicle associated pluripotent (HAP) stem cells jump from transplanted whiskers to pelage follicles and stimulate hair growth.
Obara K, Reynoso J, Hamada Y, Aoki Y, Kubota Y, Masaki N, Amoh Y, Hoffman RM. Obara K, et al. Sci Rep. 2022 Dec 7;12(1):21174. doi: 10.1038/s41598-022-25383-z. Sci Rep. 2022. PMID: 36476963 Free PMC article.
Hair-Follicle-Associated Pluripotent (HAP) Stem Cells Can Extensively Differentiate to Tyrosine-Hydroxylase-Expressing Dopamine-Secreting Neurons.
Yamane M, Takaoka N, Obara K, Shirai K, Aki R, Hamada Y, Arakawa N, Hoffman RM, Amoh Y. Yamane M, et al. Cells. 2021 Apr 10;10(4):864. doi: 10.3390/cells10040864. Cells. 2021. PMID: 33920157 Free PMC article.

See all "Cited by" articles

References

1. Hoffman R.M. The hair follicle as a gene therapy target. Nat Biothechnol 18, 20, 2000 - PubMed
1. Oshima H., Rochat A., Kedzia C., Kobayashi K., and Barrandon Y. Morphogenesis and renewal of hair follicles from adult multipotent stem cells. Cell 104, 233, 2001 - PubMed
1. Cotsarelis G., Sun T.T., and Lavker R.M. Label-retaining cells reside in the bulge area of pilosebaceous unit: implications for follicular stem cells, hair cycle, and skin carcinogenesis. Cell 61, 1329, 1990 - PubMed
1. Li L., Mignone J., Yang M., Matic M., Penman S., Enikolopov G., et al. . Nestin expression in hair follicle sheath progenitor cells. Proc Natl Acad Sci U S A 100, 9958, 2003 - PMC - PubMed
1. Amoh Y., Li L., Yang M., Moossa A.R., Katsuoka K., Penman S., et al. . Nascent blood vessels in the skin arise from nestin-expressing hair-follicle cells. Proc Natl Acad Sci U S A 101, 13291, 2004 - PMC - PubMed

Publication types

Actions

MeSH terms

Actions
Actions
Actions
Actions
Actions
Actions
Actions
Actions
Actions
Actions
Actions

Substances

Actions
Actions
Actions

Grants and funding

NS086217/NS/NINDS NIH HHS/United States

LinkOut - more resources

Full Text Sources
Other Literature Sources
- scite Smart Citations
Miscellaneous
- NCI CPTAC Assay Portal

Save citation to file

Email citation

Add to Collections

Add to My Bibliography

Your saved search

Create a file for external citation management software

Your RSS Feed

Cryopreservation of the Hair Follicle Maintains Pluripotency of Nestin-Expressing Hair Follicle-Associated Pluripotent Stem Cells

Affiliations

Cryopreservation of the Hair Follicle Maintains Pluripotency of Nestin-Expressing Hair Follicle-Associated Pluripotent Stem Cells

Authors

Affiliations

Abstract

Figures

Similar articles

Cited by

References

Publication types

MeSH terms

Substances

Grants and funding

LinkOut - more resources

Full Text Sources

Other Literature Sources

Miscellaneous

Abstract

Figures

Similar articles

Cited by

References

Publication types

MeSH terms

Substances

Related information

Grants and funding

LinkOut - more resources

Full Text Sources

Other Literature Sources

Miscellaneous