The aim of this work was to evaluate chromatin and spindle organization of buffalo and bovine in vitro matured oocytes after vitrification/warming by Cryotop and after their exposure to cryoprotectants (CP). In vitro matured oocytes were vitrified/warmed and exposed to the vitrification/warming solutions containing ethylene glycol (EG), dimethyl sulfoxide (DMSO) and sucrose as CP. Two hours after warming, oocytes were fixed and immunostained for microtubules and nuclei and examined by fluorescence microscopy. Data were analyzed by Chi Square test. A higher percentage of Telophase II stage oocytes was found in the toxicity (26 and 34% in bovine and buffalo) and the vitrification groups (13 and 7% in bovine and buffalo) compared to the control, indicating occurrence of activation. An increased percentage of oocytes with abnormal spindle and chromosome organization was found in oocytes exposed to CP (24 and 13% in bovine; 32 and 30% in buffalo respectively) and in those vitrified (26 and 31% in bovine; 26 and 29% in buffalo respectively) compared to the control (0 in bovine and 2.5 % in buffalo)

Bianca Gasparrini

E. Mariotti

Marcello Rubessa

Marina De Blasi

Salvatore Velotto

Serena Di Francesco

Italian Journal of Animal Science

English

Evelina Mariotti

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Structural changes of in vitro matured buffalo and bovine oocytes following cryopreservation

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Full Terms & Conditions of access and use can be found athttp://www.tandfonline.com/action/journalInformation?journalCode=tjas20Download by: [Southern Cross University] Date: 04 October 2017, At: 19:11Italian Journal of Animal ScienceISSN: (Print) 1828-051X (Online) Journal homepage: http://www.tandfonline.com/loi/tjas20Structural changes of in vitro matured buffalo andbovine oocytes following cryopreservationBianca Gasparrini, Serena Di Francesco, Marcello Rubessa, Salvatore Velotto,Evelina Mariotti & Marina De BlasiTo cite this article: Bianca Gasparrini, Serena Di Francesco, Marcello Rubessa, Salvatore Velotto,Evelina Mariotti & Marina De Blasi (2009) Structural changes of in vitro matured buffalo and bovineoocytes following cryopreservation, Italian Journal of Animal Science, 8:sup2, 90-92, DOI: 10.4081/ijas.2009.s2.90To link to this article:  http://dx.doi.org/10.4081/ijas.2009.s2.90Copyright 2009 Taylor & Francis Group LLCPublished online: 07 Mar 2016.Submit your article to this journal Article views: 7View related articles Structural changes of in vitro matured buffalo and bovine oocytes following cryopreservationBianca Gasparrini1, Serena Di Francesco1, Marcello Rubessa1, Salvatore Velotto2, Evelina Mariotti1, Marina De Blasi11Dipartimento di Scienze Zootecniche ed Ispezione degli Alimenti, Università di Napoli  “Federico II”, Italy2Dipartimento di Scienze del Suolo, della Pianta, dell’Ambiente e delle Produzioni Animali,  Università di Napoli “Federico II”, ItalyCorresponding author�� Bianca Gasparrini. Dipartimento di Scienze Zootecniche ed Ispezione degli Alimenti, Facoltà di Medicina Veterinaria, Università di Napoli “Federico II”. Via F. Delpino 1, 801�7 Napoli, Italy - Tel. ���� 081 2����4��4/4��1 - Fa��� ���� 081 2��2��81 - Email�� bgasparr@unina.itAbstrAct - The aim of this work was to evaluate chromatin and spindle organization of buffalo and bovine in vitro matured oocytes after vitrification/warming by Cryotop and after their e�posure to cryo-protectants (CP). In vitro matured oocytes were vitrified/warmed and e�posed to the vitrification/warming solutions containing ethylene glycol (EG), dimethyl sulfo�ide (DMSO) and sucrose as CP. Two hours after             warming, oocytes were fi�ed and immunostained for microtubules and nuclei and e�amined by fluores-cence microscopy. Data were analyzed by Chi Square test. A higher percentage of Telophase II stage oo-cytes was found in the to�icity (2�� and �4% in bovine and buffalo) and the vitrification groups (1� and 7% in bovine and buffalo) compared to the control, indicating occurrence of activation. An increased percentage of oocytes with abnormal spindle and chromosome organization was found in oocytes e�posed to CP (24 and 1�% in bovine; �2 and �0% in buffalo respectively) and in those vitrified (2�� and �1% in bovine; 2�� and 2��% in buffalo respectively) compared to the control (0 in bovine and 2.� % in buffalo).Key words: Ultrastructure, Oocyte vitrification, Buffalo, Bovine.Introduction - The progress in oocyte cryopreservation would improve domestic animal breeding by genetic selection programs. However, despite the enormous progress in embryo cryopreservation, oocyte cryopreservation still remains a demanding task in the majority of mammalian species. In particular, buf-falo oocytes are particularly sensitive to chilling injuries, because of their high intracytoplasmic lipid con-tent (Gasparrini et al., 200��). One of the most successful ultrarapid vitrification techniques is the Cryotop           vitrification (CTV) that has resulted in e�cellent survival and developmental rates with human and bovine Metaphase II (MII) oocytes (Kuwayama et al., 200�). This method has also been successfully used for cryopreservation of ovine (Succu et al., 2008), pig (Fujihira et al., 200�), and buffalo oocytes (Gasparrini et al., 2007). However, despite the improvement in survival and cleavage rates, development into blastocysts is still poor, probably because of ultrastructural and physiological changes that occur as a consequence of vitrification. It is known that vitrification causes several ultrastructural (Hyttel et al., 2000) and structural alterations, including damages of the meiotic spindle apparatus in the oocyte of several species (Rho et al, 2002; Rojas et al., 2004; Succu et al., 2008). The aim of this work was to evaluate chromosome and spindle organization of buffalo and bovine in vitro matured oocytes after vitrification/warming by Cryotop and after their e�posure to cryoprotectants (CP).Material and methods - Abattoir-derived cumulus–oocyte comple�es (COCs) with a compact, non-atretic cumulus and a homogeneous cytoplasm were matured in vitro according to our standard procedures (Gaspar-Ital.J.anIm.ScI. vol. 8 (Suppl. 2), 90-92, 20090007_240_Genetics_II_bozza.indd   90 20-05-2009   11:13:44Downloaded by [Southern Cross University] at 19:11 04 October 2017 rini et al., 200��, 2008). After in vitro maturation (IVM), COCs were mechanically stripped of their cumulus cells by gentle pipetting in Hepes-buffered TCM 1���� (H1����) supplemented with 10% fetal calf serum (FCS). All media for vitrification/warming were made in a base solution consisting of H1���� medium supplemented with 20% FCS, and all equilibration and dilution steps were carried out at room temperature. The denuded oocytes were vitrified by the Cryotop method, previously described (Kuwayama and Kato, 2000). Briefly, oo-cytes were equilibrated in 10% EG and 10% DMSO for � min, transferred into 20% EG and 20% DMSO in TCM 1���� with 20% FCS �0.� M sucrose, loaded on Cryotops, and plunged into liquid nitrogen within 2� s. For warming, the Cryotop strip was immersed directly into 1 ml of 1.2� M sucrose solution for 1 min, and recovered oocytes were then e�posed to decreasing concentrations of sucrose (0.��2 M, 0.42 M, and 0.�1 M) for �0 s each. In order to test CP to�icity, COCs were e�posed to the vitrification and warming solutions. In both cases, oocytes were rinsed and allocated to IVM drops for 2 h.To evaluate the status of the meiotic spindle 2 h                     after warming, oocytes were fi�ed and immunostained for microtubules using a method previously described (Messinger and Albertini, 1����1), stained for nuclei with Hoechst and e�amined by fluorescence microscopy. Fresh in vitro matured oocytes were fi�ed and stained as control. Data were analyzed by Chi Square test.results and conclusions - The results of vitrification and e�posure to CP (to�icity) on bovine and buffalo IVM oocytes are shown in Table 1 and 2, respectively. The most interesting finding of the pres-ent study was the occurrence of spontaneous parthenogenetic activation, indicated by the presence of oocytes in Telophase stage (TII). It was previously reported that vitrification or e�posure to CP causes a transient increase in intracellular calcium concentration in mouse oocytes that is comparable to the calcium rise triggered by sperm penetration (Larman et al., 200��).Recently, high rates of parthenogenetic activation were reported in pig oocytes following vitrification but not following e�posure to CP (Somfai et al., 200��). Parthenogenetic activation also occurred in ovine oocytes e�posed to CP and, to a greater e�tent, to vitrification (Succu et al., 2008). An une�pected datum of our study was the evidence of a significantly higher percentage of spontaneously activated oocytes in the to�icity group compared to the vitrification group in both species. We speculate that the lower activation observed in the vitrification group may be referred to the slowing down of the metabolic activity subse-quent to thermal shock, and hence that activation after vitrification may occur later than 2 h post-warm-ing. To confirm this hypothesis, the same assessment needs to be carried out in oocytes fi�ed at later times post-warming. The other conclusion of this study is that the e�posure of oocytes to CP causes damages to the meiotic spindle and chromosome organization similar to those induced by the whole vitrification pro-Table 1.  Effect of vitrification and exposure to cryoprotectants (toxicity) on bovine IVM oocytes, spindle and chromosome organization. Maturation rate on total  number of oocytesSpindle configuration and chromosome organization  in MII oocytesNon matured oocytesTIIn (%)MIIn (%)Spindle configurationn (%)Chromosome organizationn (%)Groups n normal abnormal absent normal abnormalcontrol 112(13)a0(0)A7(87)A75(5)A0(0)A4(5)a7(100)A0(0)Atoxicity 1018(8)aA26(26)Bb67(66)B4(73)Ba16(24)B2(3)A58(87)Ba(13)Bavitrification 1112(26)bB14 (13)Ba68(61)B38(56)Bb18(26)B12(18)bB47(6)Bb21(31)Bba,bValues with different superscripts within columns are significantly different, P<0.05;  A,BValues with different superscripts within columns are significantly different, P<0.01.Ital.J.anIm.ScI. vol. 8 (Suppl. 2), 90-92, 2009 1proc. 18th nat. congr. aSpa, palermo, Italy007_240_Genetics_II_bozza.indd   91 20-05-2009   11:13:45Downloaded by [Southern Cross University] at 19:11 04 October 2017 tocol. The damages to the meiotic spindle and DNA fragmentation may lead to aneuploidy incompatible with subsequent embryo development and account for the poor embryo development currently recorded. The evidence of these structural alterations provides the basis for developing new strategies to improve the efficiency of cryopreservation in bovine and buffalo species.references - fujihira�� T., Nagai, H., Fukui, Y., 200�. Relationship between equilibration times and the      presence of cumulus cells, and effect of ta�ol treatment for vitrification of in vitro matured porcine oocytes. Cryobio-logy. �1������-�4�. Gasparrini�� B., Boccia, L., Marchandise, J., Di Palo, R., George, F., Donnay, I., Zicarelli, L., 200��. Enrichment of in vitro maturation medium for buffalo (Bubalus bubalis) oocytes with thiol compounds�� effects of cystine on glutathione synthesis and embryo development. Theriogenology. �����27�-87. Gasparrini�� B., Attanasio, L., De Rosa, A., Monaco, E., Di Palo, R., Campanile, G., 2007. Cryopreservation of in vitro matured buffalo (Bu-balus bubalis) oocytes by minimum volumes vitrification methods. Anim. Reprod. Sci. ��8�����-�42. Gasparrini�� B., Monaco, E., Boccia, L., De Rosa, A., Attanasio, L., Killian, G., 2008. Effect of osteopontin on in vitro embryo development in cattle. �4th Annual Conference of the International Embryo Transfer Society, �-�� January 2008. Reprod. Fert. Develop. 20��180. Hyttel�� P., Vajta, G., Callesen, H., 2000. Vitrification of bovine oocytes with the open pulled straw method�� ultrastructural consequences. Mol. Reprod. Dev. �����80-88. Kuwayama, M., Kato, O., 2000. All-round vitrification method for human oocytes and embryos. J. Assist. Reprod. Genet. 17��477. Kuwayama, M., Vajta, G., Kato, O., Leibo, S.P., 200�. Highly efficient vitrification method for cryopreservation of human oocytes. Reprod. Biomed. 11���00-�08. Larman�� M.G., Sheehan, C.B., Gardner, D.K., 200��. Calcium free vitrification reduces cryoprotectant-induced zona pellucida hardening and increases fertilization rates in mouse oocytes. Reproduction. 1�1����-��1. Messinger, S.M., Albertini, D.F., 1����1. Centrosome and microtubule dynamics during meiotic progres-sion in the mouse oocyte. J. Cell Sci. 100��28��-2��8. rho�� G.J., Kim, S., Yoo, J.G., Balasubramanian, S, Lee, H.J., Choe, S.Y., 2002. Microtubulin configuration and mitochondrial distribution after ultra-rapid cooling of bovine oocytes. Mol. Reprod. Dev. �����4��4-470. rojas�� C., Palomo, M.J., Albarracin, J.L., Mogas, T., 2004. Vitrification of immature and in vitro matured pig oocytes�� study of distribution of chromosomes, microtubules, and actin microfilaments. Cryobiology. 4����211-220. somfai�� T., Dinnyés, A., Sage, D., Marosán, M., Carnwath, J.W., Ozawa, M., Kikuchi, K., Niemann, H., 200��. Development to the blastocyst stage of parthenogenetically activated in vitro matured porcine oocytes after solid surface vitrification (SSV). Theriogenology. ������41�-422. succu, S., Bebbere, D., Bogliolo, L., Ariu, F., Fois, S., Leoni, G.G., Berlinguer, F., Naitana, S., Ledda, S., 2008. Vitrification of in vitro matured ovine oocytes affects in vitro pre-implantation development and mRNA abundance. Mol. Reprod. Dev. 7�����8-�4��.Table 2.  Effect of vitrification and exposure to cryoprotectants (toxicity) on buffalo IVM oocytes, spindle and chromosome organization.Maturation rate on total  number of oocytesSpindle configuration and chromosome organization  in MII oocytesNon matured oocytesTIIn (%)MIIn (%)Spindle configurationn (%)Chromosome organizationn (%)Groups n normal abnormal absent normal abnormalcontrol 010(11)0(0)aA80(8)A78(7)A2(3)A0(0)78(7)A2(3)Atoxicity 1176(5)40(34)B71(61)B48(68)B23(32)B0(0)50(70)B21(30)Bvitrification 1148(7)8(7)bA8(86)A6(70)B26(27)C3(3)70(71)B28(2)Ba,bValues with different superscripts within columns are significantly different, P<0.05; A,B,CValues with different superscripts within columns are significantly different, P<0.01.Ital.J.anIm.ScI. vol. 8 (Suppl. 2), 90-92, 20092proc. 18th nat. congr. aSpa, palermo, Italy007_240_Genetics_II_bozza.indd   92 20-05-2009   11:13:45Downloaded by [Southern Cross University] at 19:11 04 October 2017 

Structural changes of in vitro matured buffalo and bovine oocytes following cryopreservation.

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Structural changes of in vitro matured buffalo and bovine oocytes following cryopreservation.

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