Resumo
Diabetic nephropathy (DN) is a prevalent diabetic microvascular condition. It is the leading cause of kidney disease in the advanced stages. There is no currently effective treatment available. This research aimed to investigate the curative potentials of exosomes isolated from mesenchymal stem cells affecting DN. This study was performed on 70 male adult albino rats. Adult rats were randomized into seven groups: Group I: Negative control group, Group II: DN group, Group III: Balanites treated group, Group IV: MSCs treated group, Group V: Exosome treated group, Group VI: Balanites + MSCs treated group and Group VII: Balanites + exosome treated group. Following the trial period, blood and renal tissues were subjected to biochemical, gene expression analyses, and histopathological examinations. Results showed that MDA was substantially increased, whereas TAC was significantly decreased in the kidney in the DN group compared to normal health rats. Undesired elevated values of MDA levels and a decrease in TAC were substantially ameliorated in groups co-administered Balanites aegyptiacae with MSCs or exosomes compared to the DN group. A substantial elevation in TNF-α and substantially diminished concentration of IGF-1 were noticed in DN rats compared to normal health rats. Compared to the DN group, the co-administration of Balanites aegyptiacae with MSCs or exosomes substantially improved the undesirable elevated values of TNF-α and IGF-1. Furthermore, in the DN group, the mRNA expression of Vanin-1, Nephrin, and collagen IV was significantly higher than in normal healthy rats. Compared with DN rats, Vanin-1, Nephrin, and collagen IV Upregulation were substantially reduced in groups co-administered Balanites aegyptiacae with MSCs or exosomes. In DN rats, AQP1 expression was significantly lower than in normal healthy rats. Furthermore, the groups co-administered Balanites aegyptiacae with MSCs or exosomes demonstrated a substantial increase in AQP1 mRNA expression compared to DN rats.
A nefropatia diabética (ND) é uma condição microvascular diabética prevalente. É a principal causa de doença renal em estágios avançados. Atualmente, não há tratamento eficaz disponível. Esta pesquisa teve como objetivo investigar os potenciais curativos de exossomos isolados de células-tronco mesenquimais que afetam a ND. Este estudo foi realizado em 70 ratos albinos adultos machos. Ratos adultos foram randomizados em sete grupos: Grupo I: Grupo de controle negativo, Grupo II: Grupo DN, Grupo III: Grupo tratado com Balanites, Grupo IV: Grupo tratado com MSCs, Grupo V: Grupo tratado com exossomos, Grupo VI: Grupo tratado com Balanites + MSCs e Grupo VII: Balanites + grupo tratado com exossomas. Após o período experimental, o sangue e os tecidos renais foram submetidos a análises bioquímicas, de expressão gênica e exames histopatológicos. Os resultados mostraram que o MDA aumentou substancialmente, enquanto o TAC diminuiu significativamente no rim no grupo DN em comparação com ratos saudáveis normais. Valores elevados indesejados de níveis de MDA e uma diminuição no TAC foram substancialmente melhorados em grupos coadministrados Balanites aegyptiacae com MSCs ou exossomas em comparação com o grupo DN. Uma elevação substancial em TNF-α e uma concentração substancialmente diminuída de IGF-1 foram observadas em ratos DN em comparação com ratos saudáveis normais. Em comparação com o grupo DN, a coadministração de Balanites aegyptiacae com MSCs ou exossomas melhorou substancialmente os valores elevados indesejáveis de TNF-α e IGF-1. Além disso, no grupo DN a expressão de mRNA de vanina-1, nefrina e colágeno IV foi significativamente maior do que em ratos saudáveis normais. Comparado com ratos DN, Vanin-1, Nephrin e colágeno IV Upregulation foram substancialmente reduzidos em grupos co-administrados Balanites aegyptiacae com MSCs ou exossomos. Em ratos DN, a expressão de AQP1 foi significativamente menor do que em ratos saudáveis normais. Além disso, os grupos que coadministraram Balanites aegyptiacae com MSCs ou exossomos demonstraram um aumento substancial na expressão de mRNA de AQP1 em comparação com ratos DN.
Assuntos
Animais , Ratos , Nefropatias Diabéticas , Aquaporina 1 , Células-Tronco MesenquimaisResumo
Background: Canine distemper (CD) is a highly contagious viral disease caused by the canine distemper virus (CDV). In dogs, CDV infection is characterized by the presentation of systemic and/or neurological signs with viral persistence in some organs, including the central nervous system (CNS). Neurological damages resulting from CD are a defiance for veterinarians, due to occasioned clinical sequels that influence the patient quality of life. The treatment of sequelae should seek to promote the resolution or decrease of the deleterious effects that impede the patient independence. Thus, the present report aims to describe the action of antiparkinsonian medication (levodopa associated with carbidopa) administered to 3 dogs who presented neurological sequels resulting from the canine distemper. Cases: Dog 1. A 9-month-old male mixed breed; Dog 2. A 6-month-old male Shih Tzu. Dog 3. A 8-years-old bitch mixed breed. All animals were referred for neurological care because presented neurological damages after distemper involvement. Only the Dog 2 was vaccinated to CD. Dog 1 (mixed male) had severe myoclonus, lack of proprioception, decreased of muscle tonus and paralysis in both pelvic limbs, associated with a marked thoracolumbar kyphosis. Dog 2 (a puppy Shih Tzu male) presented myoclonus in PL, proprioceptive loss in thoracic and pelvic limbs, absence of withdrawal reflex in thoracic and pelvic limbs, decrease in muscle tonus in pelvic limb and increase in thoracic limb. Dog 3 (adult unneutered bitch) presented intense myoclonus, absence of proprioception, decrease in muscle tonus and paresis of pelvic limb. All patients were treated with antiparkinsonian medication (levodopa 250 mg associated with carbidopa 25 mg) with following dosages: Dog 1 received a commercially available tablet, orally once a day for 30 days, while Dogs 2 and 3 had doses calculated by extrapolation allometric. For the Dog 2 it was prescribed 0.25 mg of levodopa and 0.025 mg of carbidopa daily for 30 days. Dog 3 was treated with 1 mg of levodopa and 0.1 mg of carbidopa patient day for the same period. Thirty days after starting the treatment, the 3 patients were evaluated again, and showed improvement of the motor signs, and the treatment was maintained. At the next return (30 days): Dog 1 showed significant improvement, however, Dog 2 started to present epileptic seizures and nystagmus that were treated with levetiracetam, while the Dog 3 not returned. As Dog 1 had a better prognosis, treatment was maintained for 1 year, with the frequency being changed from 24 h x 24 h to 48 h x 48 h after 30 days and 72x72 h after another 30 days. Unfortunately, Dog 2 had a worsening of epileptic condition and died, while Dog 3 died by road-kill. Discussion: The cases reported are uncommon, because not exist information about the use of antiparksonian to treatment of neurological damages occasioned by canine distemper. Although there are emerging therapies, such as the use of mesenchymal stem cells, that can reduce these sequels, the access is still restricted to a few professionals. Thus, the use of medications for demyelinating diseases, as antiparkinsonian, may be an alternative. In fact, the three reported patients showed recovery of the motor and sensorial damages observed, which corroborates with the possibility of a new treatment using antiparkinsonian or other drugs to demyelinating diseases.
Assuntos
Animais , Cães , Carbidopa/administração & dosagem , Levodopa/administração & dosagem , Transtornos Parkinsonianos/veterinária , Cinomose/terapia , Antiparkinsonianos/uso terapêuticoResumo
Infertility is one of the most prevalent health disorders in reproductive-age males and females. Ficus carica (Fc), an herbal plant, has been used traditionally for the treatment of different diseases such as infertility especially in Iranian folk medicine. This study examined the effects of Fc leaf extract on the proliferation of mice spermatogonial stem cells (SSCs). Phenolic, flavonoid content, major polyphenolic compounds and antioxidant activity of the extract was evaluated respectively by Folin-Ciocateu, aluminum chloride, HPLC and the FRAP and DPPH methods. Testicular cells of neonate mice were extracted and their identity was confirmed using cytokeratin for Sertoli and Oct-4, CDHI and PLZF for SSCs. Effects of Fc (0.0875, 0.175, 0.35, 0.71 and 1.42 mg/ml) was evaluated at third, 7th, 9th and 14th days of culture by colony assay. The expression of the Mvh, GFRα1 and Oct-4 genes and the viability and proliferation of cultured cells was assessed at the end of the culture period. The extract has a rich phenolic and flavonoid content such as Rutin, Psoralen, Bergapten and Caffeoylmalic acid using HPLC analysis. It also had a potent reducing and radical scavenging activity. Morphology of colonies was similar in all groups. Higher viability, proliferation, colony number and diameter of SSCs was seen in the presence of Fc leaf extract in a dosedependent manner so that higher number and diameter of colonies were observed in two higher doses of 0.71 and 1.42 mg/ml, separately for each time point relative to other groups. The Mvh, Oct-4 and GFRα1 genes expression had no significant differences between groups. It seems that Fc leaf extract not only had no any cytotoxic effects on the viability and proliferation of SSCs but also support their stemness state. So, this culture system can be employed for enrichment of germ stem cells for use in clinical applications.(AU)
Assuntos
Animais , Camundongos , Extratos Vegetais/efeitos adversos , Ficus/efeitos adversos , Camundongos/embriologia , Citotoxicidade Imunológica , Células-Tronco Germinativas Adultas/citologiaResumo
The creation of a genetic resource bank of avian species aims to prevent the decline and fragmentation of wild bird populations, which in turn lead to the loss of genetic diversity and, in more serious cases, the extinction of the most threatened species. In order for the collected genetic material to be stored in a bank and useful when necessary, it is essential to improve the technique ensuring its effectiveness. Thus, our study used feather follicle cells from the domestic gallus species to standardize the technique of cell culture and subsequent cryopreservation. This study aimed to establish a protocol, in vitro, of isolation and primary culture of somatic cells derived from the feather follicle, with the purpose of establishing a cell lineage, and evaluate its viability for the biobank formation. Developing feathers of gallus domesticus were collected at 12, 21 and 34 days of age. The feathers were morphologically analyzed and then we selected the region of the calamus due to the presence of pulp for cell culture and cryopreservation. The results showed that it is possible to find cells with distinct morphology; cells in elliptical shape with central nucleus also in elliptical shape, cells with shape and round nucleus, cells compatible with the fibers of the barbules, cell agglomerates and cells adhered to the bottom of the plate with fibroblastatoid shape. After 24 hours of culture there was the presence of primary culture with 80% of confluence and after cryopreservation the average viability after freezing was 68.8%, with cellular morphologies being maintained. Therefore, we proved the isolation of somatic cells from the follicle of birds feathers, suggesting that this is a source of great value, viable and effective for obtaining biological material for the elaboration of a biobank.
Assuntos
Animais , Embrião de Galinha , Galinhas/genética , Plumas , Células-Tronco AdultasResumo
The creation of a genetic resource bank of avian species aims to prevent the decline and fragmentation of wild bird populations, which in turn lead to the loss of genetic diversity and, in more serious cases, the extinction of the most threatened species. In order for the collected genetic material to be stored in a bank and useful when necessary, it is essential to improve the technique ensuring its effectiveness. Thus, our study used feather follicle cells from the domestic gallus species to standardize the technique of cell culture and subsequent cryopreservation. This study aimed to establish a protocol, in vitro, of isolation and primary culture of somatic cells derived from the feather follicle, with the purpose of establishing a cell lineage, and evaluate its viability for the biobank formation. Developing feathers of gallus domesticus were collected at 12, 21 and 34 days of age. The feathers were morphologically analyzed and then we selected the region of the calamus due to the presence of pulp for cell culture and cryopreservation. The results showed that it is possible to find cells with distinct morphology; cells in elliptical shape with central nucleus also in elliptical shape, cells with shape and round nucleus, cells compatible with the fibers of the barbules, cell agglomerates and cells adhered to the bottom of the plate with fibroblastatoid shape. After 24 hours of culture there was the presence of primary culture with 80% of confluence and after cryopreservation the average viability after freezing was 68.8%, with cellular morphologies being maintained. Therefore, we proved the isolation of somatic cells from the follicle of birds feathers, suggesting that this is a source of great value, viable and effective for obtaining biological material for the elaboration of a biobank.(AU)
Assuntos
Animais , Galinhas/genética , Embrião de Galinha , Plumas , Células-Tronco AdultasResumo
Pluripotent stem cells have been studied as source of cells for regenerative medicine and acquire or genetic diseases, as an innovative therapy. Most tissues have stem cells populations, however in few quantities or impossible to be used during adult life, which lead to scientists look for new sources. Thus, this study aimed to analyze the presence of pluripotent cells in the uterus and placenta, following up non-pregnant, pregnant (begin, middle, and final), and postpartum periods in dogs. The uteri were obtained from social castration programs for population control in Pirassununga, Sao Paulo, Brazil. It was collected 20 uteri at different stages. The samples were fixed and processed for immunohistochemical analysis of NANOG, OCT4 and SOX2 expression, knowing as pluripotent stem cells makers. Our results showed positive expression for NANOG, OCT4 and SOX2 in all stages of gestation and nonpregnant uterus; however, we highlight some quantitative different between stages. OCT4 showed more expression in non-pregnant uterus than NANOG and SOX2, and its expression increased in pregnant uterus. In pregnant uterus there was more expression of NANOG than OCT4 and SOX2. Interesting, no difference was found between these markers in the other periods. In conclusion, it was possible to identify pluripotent stem cells in all periods in dog placenta and uterus, however during the early stage of pregnancy we observed more pluripotent stem cells than in all the others periods confirming the high plasticity and regeneration capacity of the uterine tissue.
Assuntos
Feminino , Animais , Cães , Cães/fisiologia , Células-Tronco Pluripotentes , PlacentaçãoResumo
Pluripotent stem cells have been studied as source of cells for regenerative medicine and acquire or genetic diseases, as an innovative therapy. Most tissues have stem cells populations, however in few quantities or impossible to be used during adult life, which lead to scientists look for new sources. Thus, this study aimed to analyze the presence of pluripotent cells in the uterus and placenta, following up non-pregnant, pregnant (begin, middle, and final), and postpartum periods in dogs. The uteri were obtained from social castration programs for population control in Pirassununga, Sao Paulo, Brazil. It was collected 20 uteri at different stages. The samples were fixed and processed for immunohistochemical analysis of NANOG, OCT4 and SOX2 expression, knowing as pluripotent stem cells makers. Our results showed positive expression for NANOG, OCT4 and SOX2 in all stages of gestation and nonpregnant uterus; however, we highlight some quantitative different between stages. OCT4 showed more expression in non-pregnant uterus than NANOG and SOX2, and its expression increased in pregnant uterus. In pregnant uterus there was more expression of NANOG than OCT4 and SOX2. Interesting, no difference was found between these markers in the other periods. In conclusion, it was possible to identify pluripotent stem cells in all periods in dog placenta and uterus, however during the early stage of pregnancy we observed more pluripotent stem cells than in all the others periods confirming the high plasticity and regeneration capacity of the uterine tissue.(AU)
Assuntos
Animais , Feminino , Cães , Cães/fisiologia , Células-Tronco Pluripotentes , PlacentaçãoResumo
Bone tissue repair remains a challenge in tissue engineering. Currently, new materials are being applied and often integrated with live cells and biological scaffolds. The fibrin biopolymer (FBP) proposed in this study has hemostatic, sealant, adhesive, scaffolding and drug-delivery properties. The regenerative potential of an association of FBP, biphasic calcium phosphate (BCP) and mesenchymal stem cells (MSCs) was evaluated in defects of rat femurs. Methods: Adult male Wistar rats were submitted to a 5-mm defect in the femur. This was filled with the following materials and/or associations: BPC; FBP and BCP; FBP and MSCs; and BCP, FBP and MSCs. Bone defect without filling was defined as the control group. Thirty and sixty days after the procedure, animals were euthanatized and subjected to computed tomography, scanning electron microscopy and qualitative and quantitative histological analysis. Results: It was shown that FBP is a suitable scaffold for bone defects due to the formation of a stable clot that facilitates the handling and optimizes the surgical procedures, allowing also cell adhesion and proliferation. The association between the materials was biocompatible. Progressive deposition of bone matrix was higher in the group treated with FBP and MSCs. Differentiation of mesenchymal stem cells into osteogenic lineage was not necessary to stimulate bone formation. Conclusions: FBP proved to be an excellent scaffold candidate for bone repair therapies due to application ease and biocompatibility with synthetic calcium-based materials. The satisfactory results obtained by the association of FBP with MSCs may provide a more effective and less costly new approach for bone tissue engineering.(AU)
Assuntos
Animais , Ratos , Biopolímeros , Matriz Óssea , Fibrina , Células-Tronco Mesenquimais , Produtos BiológicosResumo
There is a growing interest in the study of unspecialized mesenchymal stem cells, for there are still some discussions about their in vitro behavior. Regenerative medicine is a science undergoing improvement which develops treatments as cell therapy using somatic stem cells. In several studies, adipose tissue is presented as a source of multipotent adult cells that has several advantages over other tissue sources. This study aimed to characterize and evaluate the tagging of mesenchymal stem cells from the agoutis adipose tissue (Dasyprocta prymonolopha), with fluorescent intracytoplasmic nanocrystals. Fibroblast cells were observed, plastic adherent, with extended self-renewal, ability to form colonies, multipotency by differentiation into three lineages, population CD90 + and CD45 - expression, which issued high red fluorescence after the tagging with fluorescent nanocrystals by different paths and cryopreserved for future use. It is possible to conclude that mesenchymal stem cells from agouti adipose tissue have biological characteristics and in vitro behavior that demonstrate its potential for use in clinical tests.(AU)
Há um interesse crescente no estudo das células estaminais mesenquimais, não especializadas, pois ainda existem algumas discussões sobre seu comportamento in vitro. A medicina regenerativa é uma ciência em fase de crescimento que desenvolve tratamentos como terapia celular utilizando células estaminais somáticas. Em vários estudos, o tecido adiposo é apresentado como uma fonte de células adultas multipotentes que tem várias vantagens em relação a outras fontes de tecido. Este estudo teve como objetivo caracterizar e avaliar a marcação de células estaminais mesenquimais do tecido adiposo de cutias (Dasyprocta prymnolopha) com nanocristais intracitoplasmáticos fluorescentes. Observaram-se células fibroblásticas, aderentes ao plástico, com autorrenovação prolongada, capacidade de formar colônias, diferenciação em três linhagens, população CD90 + e expressão CD45, que emitiram alta fluorescência vermelha após a marcação com nanocristais fluorescentes por diferentes vias, e criopreservadas para uso futuro. É possível concluir que as células estaminais mesenquimais do tecido adiposo de cutias têm características biológicas e comportamentos in vitro que demonstram seu potencial para uso em testes clínicos.(AU)
Assuntos
Animais , Tecido Adiposo/citologia , Imunofenotipagem/veterinária , Medicina Regenerativa/métodos , Nanopartículas , Células-Tronco Mesenquimais , Dasyproctidae/genéticaResumo
There is a growing interest in the study of unspecialized mesenchymal stem cells, for there are still some discussions about their in vitro behavior. Regenerative medicine is a science undergoing improvement which develops treatments as cell therapy using somatic stem cells. In several studies, adipose tissue is presented as a source of multipotent adult cells that has several advantages over other tissue sources. This study aimed to characterize and evaluate the tagging of mesenchymal stem cells from the agoutis adipose tissue (Dasyprocta prymonolopha), with fluorescent intracytoplasmic nanocrystals. Fibroblast cells were observed, plastic adherent, with extended self-renewal, ability to form colonies, multipotency by differentiation into three lineages, population CD90 + and CD45 - expression, which issued high red fluorescence after the tagging with fluorescent nanocrystals by different paths and cryopreserved for future use. It is possible to conclude that mesenchymal stem cells from agouti adipose tissue have biological characteristics and in vitro behavior that demonstrate its potential for use in clinical tests.(AU)
Há um interesse crescente no estudo das células estaminais mesenquimais, não especializadas, pois ainda existem algumas discussões sobre seu comportamento in vitro. A medicina regenerativa é uma ciência em fase de crescimento que desenvolve tratamentos como terapia celular utilizando células estaminais somáticas. Em vários estudos, o tecido adiposo é apresentado como uma fonte de células adultas multipotentes que tem várias vantagens em relação a outras fontes de tecido. Este estudo teve como objetivo caracterizar e avaliar a marcação de células estaminais mesenquimais do tecido adiposo de cutias (Dasyprocta prymnolopha) com nanocristais intracitoplasmáticos fluorescentes. Observaram-se células fibroblásticas, aderentes ao plástico, com autorrenovação prolongada, capacidade de formar colônias, diferenciação em três linhagens, população CD90 + e expressão CD45, que emitiram alta fluorescência vermelha após a marcação com nanocristais fluorescentes por diferentes vias, e criopreservadas para uso futuro. É possível concluir que as células estaminais mesenquimais do tecido adiposo de cutias têm características biológicas e comportamentos in vitro que demonstram seu potencial para uso em testes clínicos.(AU)
Assuntos
Animais , Tecido Adiposo/citologia , Imunofenotipagem/veterinária , Medicina Regenerativa/métodos , Nanopartículas , Células-Tronco Mesenquimais , Dasyproctidae/genéticaResumo
Background:Bone tissue repair remains a challenge in tissue engineering. Currently, new materials are being applied and often integrated with live cells and biological scaffolds. The fibrin biopolymer (FBP) proposed in this study has hemostatic, sealant, adhesive, scaffolding and drug-delivery properties. The regenerative potential of an association of FBP, biphasic calcium phosphate (BCP) and mesenchymal stem cells (MSCs) was evaluated in defects of rat femurs.Methods:Adult male Wistar rats were submitted to a 5-mm defect in the femur. This was filled with the following materials and/or associations: BPC; FBP and BCP; FBP and MSCs; and BCP, FBP and MSCs. Bone defect without filling was defined as the control group. Thirty and sixty days after the procedure, animals were euthanatized and subjected to computed tomography, scanning electron microscopy and qualitative and quantitative histological analysis.Results:It was shown that FBP is a suitable scaffold for bone defects due to the formation of a stable clot that facilitates the handling and optimizes the surgical procedures, allowing also cell adhesion and proliferation. The association between the materials was biocompatible. Progressive deposition of bone matrix was higher in the group treated with FBP and MSCs. Differentiation of mesenchymal stem cells into osteogenic lineage was not necessary to stimulate bone formation.Conclusions:FBP proved to be an excellent scaffold candidate for bone repair therapies due to application ease and biocompatibility with synthetic calcium-based materials. The satisfactory results obtained by the association of FBP with MSCs may provide a more effective and less costly new approach for bone tissue engineering.(AU)
Assuntos
Animais , Ratos , Biopolímeros/uso terapêutico , Regeneração Óssea , Adesivo Tecidual de Fibrina/uso terapêutico , Células-TroncoResumo
Besides having medical applications, comparative studies on reproductive biology are very useful, providing, for instance, essential knowledge for basic, conservation and biotechnological research. In order to maintain the reproductive potential and the survival of all vertebrate species, both sperm and steroid production need to occur inside the testis. From the approximately fifty thousand vertebrate species still alive, very few species are already investigated; however, our knowledge regarding Sertoli cell biology is quite good. In this regard, it is already known that since testis differentiation the Sertoli cells are the somatic cells in charge of supporting and orchestrating germ cells during development and full spermatogenesis in adult animals. In the present review, we highlight key aspects related to Sertoli cell biology in vertebrates and show that this key testis somatic cell presents huge and intrinsic plasticity, particularly when cystic (fish and amphibians) and non-cystic (reptiles, birds and mammals) spermatogenesis is compared. In particular, we briefly discuss the main aspects related to Sertoli cells functions, interactions with germ cells, Sertoli cells proliferation and efficiency, as well as those regarding spermatogonial stem cell niche regulation, which are crucial aspects responsible for the magnitude of sperm production. Most importantly, we show that we could greatly benefit from investigations using different vertebrate experimental models, mainly now that there is a big concern regarding the decline in human sperm counts caused by a multitude of factors.
Assuntos
Células de Sertoli/classificação , Espermatogênese , Vertebrados/classificação , BiotecnologiaResumo
Besides having medical applications, comparative studies on reproductive biology are very useful, providing, for instance, essential knowledge for basic, conservation and biotechnological research. In order to maintain the reproductive potential and the survival of all vertebrate species, both sperm and steroid production need to occur inside the testis. From the approximately fifty thousand vertebrate species still alive, very few species are already investigated; however, our knowledge regarding Sertoli cell biology is quite good. In this regard, it is already known that since testis differentiation the Sertoli cells are the somatic cells in charge of supporting and orchestrating germ cells during development and full spermatogenesis in adult animals. In the present review, we highlight key aspects related to Sertoli cell biology in vertebrates and show that this key testis somatic cell presents huge and intrinsic plasticity, particularly when cystic (fish and amphibians) and non-cystic (reptiles, birds and mammals) spermatogenesis is compared. In particular, we briefly discuss the main aspects related to Sertoli cells functions, interactions with germ cells, Sertoli cells proliferation and efficiency, as well as those regarding spermatogonial stem cell niche regulation, which are crucial aspects responsible for the magnitude of sperm production. Most importantly, we show that we could greatly benefit from investigations using different vertebrate experimental models, mainly now that there is a big concern regarding the decline in human sperm counts caused by a multitude of factors.(AU)
Assuntos
Células de Sertoli/classificação , Vertebrados/classificação , Espermatogênese , BiotecnologiaResumo
O objetivo do trabalho foi avaliar o efeito do escore da condição corporal (ECC) materno sobre a capacidade de isolamento, expansão e caracterização de células-tronco mesenquimais (CTMs) derivadas do cordão umbilical de fetos caprinos. Para tanto, dezenove cabras mestiças adultas, pluríparas foram agrupadas de acordo com o ECC, atribuindo-se um escore de 1-5, (GB) grupo baixo com menor ECC, (2,3±0,1, GB, n = 9) e (GA) grupo alto com maior ECC (2,9±0,1, GA, n = 10). Durante o parto, fragmentos do cordão umbilical foram coletados e cultivados in vitro e avaliados a taxa de proliferação celular. Nenhum efeito significativo do ECC foi encontrado para os parâmetros considerados.
The objective of this study was to evaluate the effect of the maternal body condition score (ECC) on the ability to isolate, expand and characterize mesenchymal stem cells (MTCs) derived from the umbilical cord of goat fetuses. Nineteen crossbred adult crossbred goats were grouped according to ECC, giving a score of 1-5 (GB) low group with lower ECC, (2.3±0.1, GB, n = 9 ) and (GA) high group with higher ECC (2.9±0.1, GA, n = 10). During delivery, umbilical cord fragments were collected and cultured in vitro and the rate of cell proliferation was evaluated. No significant effect of ECC was found for the parameters considered.
Assuntos
Feminino , Animais , Células-Tronco/fisiologia , Ruminantes , Técnicas In Vitro/métodos , Técnicas In Vitro/veterinária , Cordão UmbilicalResumo
O objetivo do trabalho foi avaliar o efeito do escore da condição corporal (ECC) materno sobre a capacidade de isolamento, expansão e caracterização de células-tronco mesenquimais (CTMs) derivadas do cordão umbilical de fetos caprinos. Para tanto, dezenove cabras mestiças adultas, pluríparas foram agrupadas de acordo com o ECC, atribuindo-se um escore de 1-5, (GB) grupo baixo com menor ECC, (2,3±0,1, GB, n = 9) e (GA) grupo alto com maior ECC (2,9±0,1, GA, n = 10). Durante o parto, fragmentos do cordão umbilical foram coletados e cultivados in vitro e avaliados a taxa de proliferação celular. Nenhum efeito significativo do ECC foi encontrado para os parâmetros considerados.(AU)
The objective of this study was to evaluate the effect of the maternal body condition score (ECC) on the ability to isolate, expand and characterize mesenchymal stem cells (MTCs) derived from the umbilical cord of goat fetuses. Nineteen crossbred adult crossbred goats were grouped according to ECC, giving a score of 1-5 (GB) low group with lower ECC, (2.3±0.1, GB, n = 9 ) and (GA) high group with higher ECC (2.9±0.1, GA, n = 10). During delivery, umbilical cord fragments were collected and cultured in vitro and the rate of cell proliferation was evaluated. No significant effect of ECC was found for the parameters considered.(AU)
Assuntos
Animais , Feminino , Ruminantes , Células-Tronco/fisiologia , Técnicas In Vitro/veterinária , Técnicas In Vitro/métodos , Cordão UmbilicalResumo
Purpose: To evaluate the effects of rotator cuff muscle regeneration in sheep and establish an experimental model for the use of autologous stem cells as a treatment option for tendon injuries. Methods: Infrared muscle tenotomies and Penrose drain implantation were performed on 12 shoulders of six clinically healthy adult sheep. After 60 days, the tendons were submitted to tissue repair, drainage removal, and divided into two groups according to the use of autologous stromal stem cells for treatment. Muscle regeneration was performed by biopsy on days 14 and 34 after repair. Results: The treatment group with cell therapy showed neovascularization and expressive regeneration. Complete regeneration of the muscle pattern did not occur in any sample although some muscle gain was obtained in the group 1 samples at 34 days after repair and introduction of stem cells. Fatty infiltration of these samples from group 1 at 34 days was less intense than that in samples from group 2 at 34 days after repair without the introduction of autologous precursor cells. Conclusion: The sheep proved to be a good experimental model to assist in the development of research on muscle regeneration and the autologous manipulation of stem cells as a therapeutic option.(AU)
Assuntos
Animais , Ovinos , Regeneração Tecidual Guiada , Músculos , Tendões/anormalidades , Células-TroncoResumo
A clonagem por transferência nuclear de células somáticas consiste em uma atraente ferramenta para a conservação e multiplicação de espécies. A eficiência desta biotécnica depende da obtenção e seleção de células doadoras de núcleo derivadas da pele de indivíduos de interesse. Em alguns mamíferos encontrados em regiões de difícil acesso ou distantes de laboratórios especializados, o armazenamento a 4°C de tecidos somáticos da pele seria uma alternativa para a conservação do material genético desses animais. Contudo, o emprego desta técnica depende de alguns fatores, como os períodos e as condições de armazenamento a 4°C das amostras, os quais podem influenciar na recuperação das células após cultivo in vitro dos tecidos. Em mamíferos domésticos, estudos têm mostrado variações quanto ao período de estocagem e a presença de meio nutritivo. Já em mamíferos silvestres, apenas são relatados o uso da refrigeração como ferramenta de transporte em curto prazo. Assim, o objetivo desta revisão é apresentar as diferentes condições de armazenamento a 4°C de tecidos somáticos, evidenciando a importância dessa técnica para a conservação da biodiversidade.(AU)
Cloning by somatic cell nuclear transfer is an attractive tool for conservation and multiplication of species. The efficiency of this biotechnique depends on the obtaining and selection of nucleus donor cells derived from the skin of individuals of interest. In some mammals found in regions difficult to access or distant from specialized laboratories, the storage at 4°C of somatic tissues of the skin would be an alternative for the conservation of the genetic material of these animals. Nevertheless, the use of this technique depends on some factors, such as periods and storage conditions at 4°C of the samples, which may influence the recovery of the cells after tissue culture in vitro. In domestic mammals, studies have shown variations regarding the period of storage and the presence of nutrient medium. Already, in wild mammals, only is related the use of refrigeration as transportation tool in the short term. Thus, the aim of this review is to present the different conditions of storage at 4°C of somatic tissues, evidencing the importance of this technique for the conservation of biodiversity.(AU)
Assuntos
Animais , Células-Tronco Adultas/citologia , Armazenamento de Produtos , Refrigeração , Boas Práticas de Distribuição , Controle de Qualidade , Clonagem de Organismos/veterinária , Técnicas In Vitro , Mamíferos , PeleResumo
A clonagem por transferência nuclear de células somáticas consiste em uma atraente ferramenta para a conservação e multiplicação de espécies. A eficiência desta biotécnica depende da obtenção e seleção de células doadoras de núcleo derivadas da pele de indivíduos de interesse. Em alguns mamíferos encontrados em regiões de difícil acesso ou distantes de laboratórios especializados, o armazenamento a 4°C de tecidos somáticos da pele seria uma alternativa para a conservação do material genético desses animais. Contudo, o emprego desta técnica depende de alguns fatores, como os períodos e as condições de armazenamento a 4°C das amostras, os quais podem influenciar na recuperação das células após cultivo in vitro dos tecidos. Em mamíferos domésticos, estudos têm mostrado variações quanto ao período de estocagem e a presença de meio nutritivo. Já em mamíferos silvestres, apenas são relatados o uso da refrigeração como ferramenta de transporte em curto prazo. Assim, o objetivo desta revisão é apresentar as diferentes condições de armazenamento a 4°C de tecidos somáticos, evidenciando a importância dessa técnica para a conservação da biodiversidade.
Cloning by somatic cell nuclear transfer is an attractive tool for conservation and multiplication of species. The efficiency of this biotechnique depends on the obtaining and selection of nucleus donor cells derived from the skin of individuals of interest. In some mammals found in regions difficult to access or distant from specialized laboratories, the storage at 4°C of somatic tissues of the skin would be an alternative for the conservation of the genetic material of these animals. Nevertheless, the use of this technique depends on some factors, such as periods and storage conditions at 4°C of the samples, which may influence the recovery of the cells after tissue culture in vitro. In domestic mammals, studies have shown variations regarding the period of storage and the presence of nutrient medium. Already, in wild mammals, only is related the use of refrigeration as transportation tool in the short term. Thus, the aim of this review is to present the different conditions of storage at 4°C of somatic tissues, evidencing the importance of this technique for the conservation of biodiversity.
Assuntos
Animais , Armazenamento de Produtos , Boas Práticas de Distribuição , Controle de Qualidade , Células-Tronco Adultas/citologia , Refrigeração , Clonagem de Organismos/veterinária , Mamíferos , Pele , Técnicas In VitroResumo
Células-tronco são conhecidas pela característica de alto potencial de auto-renovação e podem ser classificadas segundo seu estágio de indiferenciação e perfil epigenético. Células-tronco embrionárias (CTEs) e células-tronco adultas são bastante estudadas e caracterizadas, principalmente nos modelos humano e em camundongos por apresentarem novas possibilidades tanto para a medicina regenerativa quanto para o entendimento do desenvolvimento inicial dos mamíferos. Contudo, a derivação e a manutenção de CTEs em espécies domésticas é desafiadora e apresenta resultados inconsistentes em relação à manutenção da pluripotência in vitro. Nesse contexto, a geração das células pluripotentes induzidas in vitro (células iPS ou iPSCs) é imprescindível para a geração de novas possibilidades na medicina veterinária regenerativa e reprodutiva devido à capacidade de diferenciação destas em uma variedade de outros tipos celulares, inclusive em animais. Assim, esta revisão apresenta a geração das células iPS em animais domésticos, e em especial, recentes estudos sobre as etapas necessárias para a possibilidade de geração de gametas funcionais in vitro, uma importante contribuição na correção de infertilidades, conservação de espécies ameaçadas de extinção e geração de indivíduos geneticamente superiores ou modificados para aplicações agropecuárias ou biomédicas.(AU)
Stem cells are widely known for their high potential for self-renewal, being classified according to their stage of undifferentiation and epigenetic profile. Embryonic stem cells (ES) and adult stem cells are already well studied and characterized, mainly in human and mouse models, once they present new possibilities both for regenerative medicine and for understanding the initial development of mammals. However, the derivation and maintenance of ES in domestic species is challenging and presents inconsistent results regarding maintenance of in vitro pluripotency. In this context, the derivation of in vitro induced pluripotent cells (iPS cells or iPSCs) enables new possibilities in regenerative and reproductive veterinary medicine due to their ability to differentiate into a variety of other cell types. Therefore, this review presents the generation of iPS cells in domestic animals, and focuses on recent studies on the steps necessary for the generation of functional gametes in vitro, an important contribution of stem cells aiming the correction of infertility, the conservation of species in risk of extinction and for the generation of genetically superior or modified organisms for agricultural and biomedical applications.(AU)
Assuntos
Animais , Animais Domésticos/embriologia , Animais Domésticos/genética , Células-Tronco Pluripotentes Induzidas , Técnicas In Vitro , Células GerminativasResumo
Células-tronco são conhecidas pela característica de alto potencial de auto-renovação e podem ser classificadas segundo seu estágio de indiferenciação e perfil epigenético. Células-tronco embrionárias (CTEs) e células-tronco adultas são bastante estudadas e caracterizadas, principalmente nos modelos humano e em camundongos por apresentarem novas possibilidades tanto para a medicina regenerativa quanto para o entendimento do desenvolvimento inicial dos mamíferos. Contudo, a derivação e a manutenção de CTEs em espécies domésticas é desafiadora e apresenta resultados inconsistentes em relação à manutenção da pluripotência in vitro. Nesse contexto, a geração das células pluripotentes induzidas in vitro (células iPS ou iPSCs) é imprescindível para a geração de novas possibilidades na medicina veterinária regenerativa e reprodutiva devido à capacidade de diferenciação destas em uma variedade de outros tipos celulares, inclusive em animais. Assim, esta revisão apresenta a geração das células iPS em animais domésticos, e em especial, recentes estudos sobre as etapas necessárias para a possibilidade de geração de gametas funcionais in vitro, uma importante contribuição na correção de infertilidades, conservação de espécies ameaçadas de extinção e geração de indivíduos geneticamente superiores ou modificados para aplicações agropecuárias ou biomédicas.
Stem cells are widely known for their high potential for self-renewal, being classified according to their stage of undifferentiation and epigenetic profile. Embryonic stem cells (ES) and adult stem cells are already well studied and characterized, mainly in human and mouse models, once they present new possibilities both for regenerative medicine and for understanding the initial development of mammals. However, the derivation and maintenance of ES in domestic species is challenging and presents inconsistent results regarding maintenance of in vitro pluripotency. In this context, the derivation of in vitro induced pluripotent cells (iPS cells or iPSCs) enables new possibilities in regenerative and reproductive veterinary medicine due to their ability to differentiate into a variety of other cell types. Therefore, this review presents the generation of iPS cells in domestic animals, and focuses on recent studies on the steps necessary for the generation of functional gametes in vitro, an important contribution of stem cells aiming the correction of infertility, the conservation of species in risk of extinction and for the generation of genetically superior or modified organisms for agricultural and biomedical applications.