Browse > Article
http://dx.doi.org/10.1080/19768354.2011.620624

Effect of droplet vitrification on mitochondrial membrane potential and developmental competence in two-cell mouse embryos  

Kim, Bo-Hyun (Department of Biological Science, College of Natural Sciences, Wonkwang University)
Kim, Ji-Su (National Primate Research Center, Korea Research Institute of Bioscience & Biotechnology)
Ryu, Jae-Sung (Department of Biological Science, College of Natural Sciences, Wonkwang University)
Lee, So-Hyun (Department of Biological Science, College of Natural Sciences, Wonkwang University)
Lee, Ju-Taek (Department of Biological Science, College of Natural Sciences, Wonkwang University)
Kang, Jae-Yul (H-cube Hospital)
Chang, Kyu-Tae (National Primate Research Center, Korea Research Institute of Bioscience & Biotechnology)
Choo, Young-Kug (Department of Biological Science, College of Natural Sciences, Wonkwang University)
Publication Information
Animal cells and systems / v.15, no.4, 2011 , pp. 287-294 More about this Journal
Abstract
The accelerated cooling rate associated with vitrification reduces injuries attributed to cryopreservation and improves the post-freezing developmental competence of vitrified embryos. In this study, embryos were vitrified and warmed and morphologically evaluated for their development to blastocysts. Survival rates between the fresh ($96.7%{\pm}3.8%$) and vitrified embryos ($90.7%{\pm}5.1%$) did not differ significantly (P>0.05). The mitochondrial membrane potential of fresh control cells measured by 5,5',6,6'-tetrachloro-1,1',3,3'-tetraethylbenzimidazolyl carbocyanide iodide staining was similar to that of cryoprotected and vitrified embryos. Mitochondrial staining with rhodamine 123 did not differ among the fresh, cryoprotected, and vitrified embryos. Moreover, the distribution of $H_2O_2$, assessed by 2',7'-dichlorodihydrofluorescein diacetate staining, did not differ among the groups. The results showed that the developmental rate did not differ significantly among the fresh ($87.8%{\pm}11.3%$), cryoprotected ($83.2%{\pm}7.6%$), and vitrified 2-cell embryos ($75.8%{\pm}14.2%$). The mean number of the inner cell mass (ICM), trophectoderm (TE), and apoptotic cells was counted and statistically compared, and although the number of ICM and TE was decreased in the cryoprotected and vitrified embryos, there were no significant differences among the groups (P>0.05). During the cultivation period, randomly selected blastocysts from each group were stained using either 4',6-diamidino-2-phenylindole and bisbenzimide or the terminal deoxynucleotidyl transferase mediated dUTP nick-end labeling technique. The incidence of apoptosis appeared to be almost identical in all the groups. Droplet vitrification could subsequently lead to high survival and developmental rates of cryopreserved mouse embryos.
Keywords
apoptosis; mitochondrial membrane potential; vitrification;
Citations & Related Records
Times Cited By KSCI : 1  (Citation Analysis)
Times Cited By Web Of Science : 0  (Related Records In Web of Science)
Times Cited By SCOPUS : 0
연도 인용수 순위
1 Van Blerkom J, Davis P, Mathwig V, Alexander S. 2002. Domains of high-polarized and low-polarized mitochondria may occur in mouse and human oocytes and early embryos. Hum Reprod. 17:393-406.   DOI
2 Van Blerkom J, Motta P. 1979. The Cellular Basis of Mammalian Reproduction. Baltimore (MD): Urban, Schwarzenberg. Chapter 5.
3 Yang MY, Rajamahendran R. 1999. Apoptosis in bovine oocytes and in preimplantation embryos: the role of Bcl-2 and Bax gene. Biol Reprod. 60(Suppl. 1):190 (abstract)   DOI
4 Ahn HJ, Sohn IP, Kwon HC, Park YD, Min CK. 2002. Characteristics of the cell membrane fluidity, actin fibers, and mitochondrial dysfunctions of frozen-thawed twocell mouse embryos. Mol Reprod Dev. 61:466-476.   DOI   ScienceOn
5 Arav A, Yavin S, Zeron Y, Natan D, Dekel I, Gacitua H. 2002. New trends in gametes's cryopreservation. Mol Cell Endocrinol. 187:77-81.   DOI   ScienceOn
6 Crossarizza A, Kalashnikova G, Grassilli E, Chiappelli F, Salviolo S, Capri M, Barbieri D, Troiano L, Monti D, Franceschi C. 1994. Mitochondrial modification during rat thymocyte apoptosis: A study at the single cell level. Exp Cell Res. 210:2323-2330.
7 Nasr-Esfahani MM, Johnson MH. 1991. The origin of reactive oxygen species in mouse embryos cultured in vitro. Development. 113:551-560.
8 Dedov V, Roufogalis B. 1999. Organization of mitochondria in sensory neurons. FEBS Lett. 456:171-174.   DOI   ScienceOn
9 Desai N, Blackmon H, Szeptycki J, Goldfarb J. 2007. Cryoloop vitrification of human day 3 cleavage stage embryos: post-vitrification development, pregnancy outcomes and live births. Reprod Biomed Online. 14:208- 213.   DOI   ScienceOn
10 Marti M, Grossmann M, Santalo J, Egozcue J, Ponsa M. 1997. Characteristics of actin fibers and ultrastructure of the contact regions involved in the separation of blastomeres of two-cell mouse embryos, frozen-thawed without the zona pellucida. Cryobiology. 34:94-106.   DOI   ScienceOn
11 Noda Y, Matumoto M, Umaoka Y, Tatsumiki K, Kishi J, Mori T. 1991. Involvement of superoxide radicals in the mouse 2-cell block. Mol Reprod Dev. 28:356-360.   DOI   ScienceOn
12 Liebermann J, Nawroth F, Isachenko V, Isachenko E, Rahimi G, Tucker M. 2002. Potential importance of vitrification in reproductive medicine. Biol Reprod. 167:1671-1680.
13 Kowaltowski AJ, Vercesi AE. 1999. Mitochondrial damage induced by conditions of oxidative stress. Free Radic Biol Med. 26:463-471.   DOI
14 Kuleshova LL, MacFarlane DR, Trounson AO, Shaw JM. 1999. Sugars exert a major influence on the vitrification properties of ethylene glycol-based solutions and have low toxicity to embryos and oocytes. Cryobiology. 38:119-130.   DOI   ScienceOn
15 Leem SH, Ahn EK, Heo JH. 2009. Functional classification of gene expression profiles during differentiation of mouse embryonic cells on monolayer culture. Anim Cells Syst. 13:235-245.   DOI
16 Johnson MH, Nasr-Esfahani MH. 1994. Radical solutions and culture problems: could free oxygen radical be responsible for the impaired development of preimplantation mammalian embryos in vitro? Bioessays. 16:31-38   DOI   ScienceOn
17 Desai N, Tsulaia T, Szeptycki-Lawson J, AbdeHafez F, Goldfarb J, Falcone T. 2011. Vitrification of mouse embryo-derived ICM cells: a tool for preserving embryonic stem cell potential? J Assist Reprod Genet. 28:93-99.   DOI   ScienceOn
18 Dinnyes A, Dai Y, Jiang S, Yang X. 2000. High development rates of vitrified bovine oocytes following parthenogenetic activation, in vitro fertilization, and somatic cell nuclear transfer. Biol Reprod. 63:513-518.   DOI   ScienceOn
19 Dinnyes A, Lonergan P, Fair T, Boland MP. 1999. Timing of the first cleavage post-insemination affects cryosurvival of in vitro-produced bovine blastocysts. Mol Reprod Dev. 53:318-324.   DOI   ScienceOn
20 Zhao XM, Quan GB, Zhou GB, Hou YP, Zhu SE. 2007. Conventional freezing, straw, and open-pulled straw vitrification of mouse two pronuclear (2 PN) stage embryos. Anim Biotechnol. 18:203-212.   DOI   ScienceOn
21 Zhou GB, Hou YP, Jin F, Yang QE, Yang ZQ, Quan GB, Tan HM, Zhu SE. 2005. Vitrification of mouse embryos at various stages by open-pulled straw (OPS) method. Anim Biotechnol. 16:153-163.   DOI   ScienceOn
22 Liu L, Trimarchi JR, Keefe DL. 2000. Involvement of mitochondria in oxidative stress-induced cell death in mouse zygotes. Biol Reprod. 62:1745-1753   DOI   ScienceOn
23 Reubinoff BE, Pera MF, Vajta G, Trounson AO. 2001. Effective cryopreservation of human embryonic stem cells by the open pulled straw vitrification method. Hum Reprod. 16:2187-2194.   DOI
24 Riha J, Landa V, Kneissl J, Matus J, Jindra J, Kloucek Z. 1991. Vitrification of cattle embryos by direct dropping into liquid nitrogen and embryo survival after nonsurgical transfer. Zivoc Vir. 36:113-120.
25 Saha S, Rajamahendran R, Boediono A, Sumantri C, Suzuki T. 1996. Viability of bovine blastocysts obtained after 7, 8 or 9 days of culture in vitro following vitrification and one-step rehydration. Theriogenology. 46:331-343.   DOI   ScienceOn
26 Saunders KM, Parks JE. 1999. Effects of cryopreservation procedure on the cytology and fertilization rate of in vitro-matured bovine oocytes. Biol Reprod. 61:178-187.   DOI   ScienceOn
27 Selman HA, El-Danasouri I. 2002. Pregnancies derived from vitrified human zygotes. Fertil Steril. 77:422-423.   DOI   ScienceOn
28 Thouas GA, Korfiatis NA, French AJ, Jones GH, Trounson AO. 2001. Simplified technique for differential staining of inner cell mass and trophectoderm cells of mouse and bovine blastocysts. Reprod Biomed Online. 3:25-29.   DOI   ScienceOn
29 Pfaff RT, Agca Y, Liu J, Woods EJ, Peter AT, Critser JK. 2000. Cryobiology of rat embryos I: Determination of zygote membrane permeability coefficients for water and cryoprotectants, their activation energies, and the development of improved cryopreservation methods. Biol Reprod. 63:1294-1302.   DOI   ScienceOn
30 Rall WF. 1987. Factors affecting the survival of mouse embryos cryopreserved by vitrification. Cryobiology. 24:387-402.   DOI   ScienceOn
31 Vajta G, Booth PJ, Holm P, Greve T, Callesen H. 1997. Successful vitrification of early stage bovine in vitro produced embryos with the open pulled straw (OPS) method. Cryo Lett. 18:191-195
32 Vajta G, Holm P, Kuwayama M, Booth PJ, Jacobsen H, Greve T. 1998. Open Pulled Straw (OPS) vitrification: a new way to reduce cryoinjuries of bovine ova and embryos. Mol Reprod Dev. 51:53-58.   DOI   ScienceOn
33 Vajta G, Kuwayama M. 2006. Improving cryopreservation systems. Theriogenology. 65:236-244.   DOI   ScienceOn