Open-access Establishment of a protocol for obtention of neuronal stem cells lineages from the dog olfactory epithelium

Estabelecimento de um protocolo para obtenção de linhagens de células-tronco neuronais a partir do epitélio olfatório de cães

Abstracts

A morphological and cell culture study from nasal mucosa of dogs was performed in order to establish a protocol to obtain a cell population committed to neuronal lineage, as a proposal for the treatment of traumatic and degenerative lesions in these animals, so that in the future these results could be applied to the human species. Twelve mongrel dogs of 60-day aged pregnancy were collected from urban pound dogs in São Paulo. Tissue from cribriform ethmoidal lamina of the fetuses was collected at necropsy under sterile conditions around 1h to 2h postmortem by uterine sections and sections from the fetal regions described above. Isolated cells of this tissue were added in DMEM/F-12 medium under standard conditions of incubation (5% CO², >37ºC). Cell culture based on isolated cells from biopsies of the olfactory epithelium showed rapid growth when cultured for 24 hours, showing phase-bright sphere cells found floating around the fragments, attached on culture flasks. After 20 days, a specific type of cells, predominantly ellipsoids or fusiform cells was characterized in vitro. The indirect immunofluorescence examination showed cells expressing markers of neuronal precursors (GFAP, neurofilament, oligodendrocyte, and III â-tubulin). The cell proliferation index showed Ki67 immunostaining with a trend to label cell groups throughout the apical region, while PCNA immunostaining label predominantly cell groups lying above the basal lamina. The transmission electron microscopy from the olfactory epithelium of dogs revealed cells with electron-dense cytoplasm and preserving the same distribution as those of positive cell staining for PCNA. Metabolic activity was confirmed by presence of euchromatin in the greatest part of cells. All these aspects give subsidies to support the hypothesis about resident progenitor cells among the basal cells of the olfactory epithelium, committed to renewal of these cell populations, especially neurons.

Olfactory epithelium; canine cell culture; animal stem cell


Foi realizado um estudo morfológico e por cultivo celular a partir de células provenientes da mucosa olfatória de cães, como forma de estabelecer um protocolo de cultivo, como uma proposta para o tratamento de lesões traumáticas e nervosas degenerativas nestes animais e futuramente, para que tais resultados possam ser aplicados a espécie humana. Foram utilizados doze cães sem raça definida, a termo, oriundos de castrações do Centro de Controle de Zoonoses de São Paulo. O tecido da lâmina cribiforme do etmóide dos fetos foi coletado sob necropsia, em condições estéreis, 1 a 2 horas post mortem, por meio de incisão uterina e acesso da região fetal supracitada. Depois as células isoladas desse tecido foram adicionadas em médio DMEM/F-12 sob condições padrão (5% CO2, >37ºC). As células obtidas a partir de biópsias do epitélio olfatório de cães apresentaram rápido crescimento após 24 horas de cultivo, demonstrando morfologia esférica, sendo encontradas flutuando ao redor do fragmento aderido à garrafa de cultura. Após 20 dias, foram verificados tipos celulares específicos, predominantemente elipsóides ou fusiformes, foram observadas in vitro. Sob avaliação por imunofluorescência indireta observaram-se células com expressão positiva para marcadores de precursores neuronais (GFAP, Neurofilamentos, oligodendrócitos e â-tubulina III). O índice de proliferação celular mostrou-se positivo para Ki67 com uma tendência de marcação de grupos celulares ao longo da região apical, enquanto a imunomarcação para PCNA mostrou-se predominantemente em grupos celulares residentes sobre a lâmina basal. A microscopia eletrônica de transmissão do epitélio olfatório de cães revelou células com citoplasma eletrodenso e mesma distribuição das células marcadas positivamente para PCNA. A atividade metabólica foi confirmada pela presença de eucromatina em muitas regiões celulares. Todos estes aspectos sustentam a hipotese sobre a presença de células progenitoras residentes entre as células basais do epitélio olfatório comprometidas com a renovação desse epitélio, particularmente a população de neurônios.

Epitélio olfatório; cultivo de células caninas; células-tronco animais


Establishment of a protocol for obtention of neuronal stem cells lineages from the dog olfactory epithelium

Estabelecimento de um protocolo para obtenção de linhagens de células-tronco neuronais a partir do epitélio olfatório de cães

Flávio R. AlvesI,*; Ricardo R. GuerraII; Emerson T. FiorettoIII; Juliana C. DelgadoIV; Antônio A. N. Machado JúniorI; Carlos E. AmbrósioVI; I. KerkisV; Maria A. MiglinoIV

IDisciplina Diagnóstico por Imagem, Curso de Medicina Veterinária, Universidade Federal do Piauí (UFPI), Campus Cinobelina Elvas, BR 125 Km 3, Planalto Cibrazem, Bom Jesus, PI 64900-000, Brazil

IIDepartamento de Ciências Veterinárias, Centro de Ciências Agrárias, Universidade Federal da Paraíba, Campus III, Areia, PB 58397- 000, Brazil

IIILaboratório de Biologia Celular e Estrutural, Departamento de Morfologia, Centro de Ciências Biológicas e da Saúde, Universidade Federal de Sergipe, Av. Marechal Rondon s/n, São Cristovão, SE 49100- 000, Brazil

IVDepartamento de Cirurgia, Faculdade de Medicina Veterinária e Zootecnia (FMVZ), Universidade de São Paulo, Av. Prof. Dr. Orlando Marques de Paiva 87, Cidade Universitária, São Paulo, SP 05508-270, Brazil

VLaboratório de Genética, Instituto Butantan, Av. Vital Brasil 1500, Butantan, São Paulo, SP 05503-900. 7 Departamento de Ciências Básicas, Faculdade de Zootecnia e Engenharia de Alimentos (FZEA), Universidade de São Paulo, Av. Duque de Caxias Norte 225, Campus da USP, Pirassununga, SP 13635-270

ABSTRACT

A morphological and cell culture study from nasal mucosa of dogs was performed in order to establish a protocol to obtain a cell population committed to neuronal lineage, as a proposal for the treatment of traumatic and degenerative lesions in these animals, so that in the future these results could be applied to the human species. Twelve mongrel dogs of 60-day aged pregnancy were collected from urban pound dogs in São Paulo. Tissue from cribriform ethmoidal lamina of the fetuses was collected at necropsy under sterile conditions around 1h to 2h postmortem by uterine sections and sections from the fetal regions described above. Isolated cells of this tissue were added in DMEM/F-12 medium under standard conditions of incubation (5% CO2, >37ºC). Cell culture based on isolated cells from biopsies of the olfactory epithelium showed rapid growth when cultured for 24 hours, showing phase-bright sphere cells found floating around the fragments, attached on culture flasks. After 20 days, a specific type of cells, predominantly ellipsoids or fusiform cells was characterized in vitro. The indirect immunofluorescence examination showed cells expressing markers of neuronal precursors (GFAP, neurofilament, oligodendrocyte, and III â-tubulin). The cell proliferation index showed Ki67 immunostaining with a trend to label cell groups throughout the apical region, while PCNA immunostaining label predominantly cell groups lying above the basal lamina. The transmission electron microscopy from the olfactory epithelium of dogs revealed cells with electron-dense cytoplasm and preserving the same distribution as those of positive cell staining for PCNA. Metabolic activity was confirmed by presence of euchromatin in the greatest part of cells. All these aspects give subsidies to support the hypothesis about resident progenitor cells among the basal cells of the olfactory epithelium, committed to renewal of these cell populations, especially neurons.

Index terms: Olfactory epithelium, canine cell culture, animal stem cell.

RESUMO

Foi realizado um estudo morfológico e por cultivo celular a partir de células provenientes da mucosa olfatória de cães, como forma de estabelecer um protocolo de cultivo, como uma proposta para o tratamento de lesões traumáticas e nervosas degenerativas nestes animais e futuramente, para que tais resultados possam ser aplicados a espécie humana. Foram utilizados doze cães sem raça definida, a termo, oriundos de castrações do Centro de Controle de Zoonoses de São Paulo. O tecido da lâmina cribiforme do etmóide dos fetos foi coletado sob necropsia, em condições estéreis, 1 a 2 horas post mortem, por meio de incisão uterina e acesso da região fetal supracitada. Depois as células isoladas desse tecido foram adicionadas em médio DMEM/F-12 sob condições padrão (5% CO2, >37ºC). As células obtidas a partir de biópsias do epitélio olfatório de cães apresentaram rápido crescimento após 24 horas de cultivo, demonstrando morfologia esférica, sendo encontradas flutuando ao redor do fragmento aderido à garrafa de cultura. Após 20 dias, foram verificados tipos celulares específicos, predominantemente elipsóides ou fusiformes, foram observadas in vitro. Sob avaliação por imunofluorescência indireta observaram-se células com expressão positiva para marcadores de precursores neuronais (GFAP, Neurofilamentos, oligodendrócitos e â-tubulina III). O índice de proliferação celular mostrou-se positivo para Ki67 com uma tendência de marcação de grupos celulares ao longo da região apical, enquanto a imunomarcação para PCNA mostrou-se predominantemente em grupos celulares residentes sobre a lâmina basal. A microscopia eletrônica de transmissão do epitélio olfatório de cães revelou células com citoplasma eletrodenso e mesma distribuição das células marcadas positivamente para PCNA. A atividade metabólica foi confirmada pela presença de eucromatina em muitas regiões celulares. Todos estes aspectos sustentam a hipotese sobre a presença de células progenitoras residentes entre as células basais do epitélio olfatório comprometidas com a renovação desse epitélio, particularmente a população de neurônios.

Termos de indexação: Epitélio olfatório, cultivo de células caninas, células-tronco animais.

INTRODUCTION

Adult tissue-specific stem cells have demonstrated the capacity to self-renew and functional rehabilitation of lost cells throughout life (Xiao et al. 2005, Viktorov et al. 2006, Viktorov et al. 2007). Nowadays, numerous diseases such as Parkinson's and Alzheimer's diseases have been treated using cell therapy, plus satisfactory results have been demonstrated (Bjugstad et al. 2008, Levy et al. 2008). Generating human neural stem cells for transplantation is now possible, either from embryonic stem cells (ES) or fetal brain tissue. Nevertheless, the current ethical debate about the usage of the excess of human embryos and fetal tissue (Sugarman 2008, Whittaker 2008) has encouraged the development of alternatives such as the appliance of adult somatic stem cells for cell therapy.

It has been reported that mammal olfactory epithelium (OE) consisted of olfactory receptor neurons, supporting cells, global and horizontal basal stem cells, which have been demonstrated to be responsible for replacing damaged cells (Chen et al. 2004, Jang et al. 2007). Therefore, OE has been considered to be an essential source for adult neural progenitor cells. In this regard, cultured cells resembling astrocytes and oligodendrocytes of mature rodent brain have been capable to produce a population of neurosphere forming cells (NSFCs) with characteristics that are similar to those seen in cells of the central nervous system (Chandran et al. 2004, Chen et al., 2004).

Dogs have been used as models for human age-related diseases and have gained wider interest as models for developing therapeutic strategies for human degenerative diseases, due to similarities in nervous system (de Lima et al. 2007, Yuasa et al. 2008).

We believe that due to the easy access of the OE neural progenitor cells, simply based in a biopsy of the cribriform plate of the ethmoid bone; these cells should be considered in cell therapies, like future application in human and veterinary medicine. Then, this experiment was to develop a protocol of stem cells extraction from canine olfactory epithelium without contaminations to be used in future pre clinical experiments.

MATERIALS AND METHODS

Primary cell culture. Twelve mongrel dogs 60-day pregnancy age were collected of urban pound dogs from the São Paulo City. Olfactory epithelium was obtained from each dog according to previous description (Overall & Arnold 2007). Briefly, tissue from cribriform ethmoidal lamina was collected at necropsy under sterile conditions around 1h to 2h postmortem. Olfactory epithelium was rinsed three times with sterile saline solution 0.9%, and transferred (with minimal dissection) into a 35mm Petri dish (Corning, New York, NY, USA) with 100 U/ml penicillin, 100g/ml streptomycin (Invitrogen, Cat. # 15140-122). Sections were cut into pieces of about 1mm3, and applying explants culture, the tissue was kept in culture flasks of 25cm2 (TPP, Switzerland) at 37ºC in DMEM/F-12 medium (Invitrogen, Cat. #10565-018).

Cultures were maintained under standard conditions (5% CO2, >37ºC) in DMEM/F-12 medium supplemented with 10% fetal bovine serum (FBS, HyClone, Logan, Utah, USA), and penicillin/streptomycin (1%; PAA). The procedure was approved by the Bioethical Commission of Veterinary Medicine and Animal Science Faculty of São Paulo University.

Immunohistochemistry. Samples of OE were obtained and fixed in 10% formalin for histological paraffin embedding. Blocks were sliced (3-4µm) and mounted onto silan-coated glass slides. PCNA (Proliferating Cell Nuclear Antigen) and Ki67 antigen levels were determined using PCNA (Santa Cruz Biotechnology, G1607) and ki67 (DAKOcytomation, M7240) monoclonal antibody with the slides stained according to the streptavidinbiotin staining procedure. Brieûy, after deparafûnization, the slices were heated in microwave (4 times at 100ºC) in 0.01M citrate buffer solution. After gradually cooling to room temperature, the slides were incubated for 20 minutes in a 0.3% hydrogen peroxide diluted in methanol solution. Slides were rinsed with distilled water, incubated with normal rabbit serum in order to block non-speciûc binding, and incubated with primary antibody, diluted to 1:100 in buffer solution, overnight at 4ºC. After incubation with the secondary antibody for 30 minutes, the slides then were incubated with the avidin-biotin complex for 30 minutes. Immunostaining was visualized by diaminobenzidine (stained for 8 minutes) and counterstained with hematoxylin.

Transmission electron microscopy. For electron microscopy, we followed the descriptions of the Lima et al. (2007), briefly, samples were fixed in Karnovsky solution (5% glutaraldehyde, 1% formaldehyde) in sodium cacodylate buffer (0.125M; pH 7.4) for 72h and, dehydrated in a crescent series of ethanol and, embedded in Spurr epoxy resin (ProSciTech, Queensland). Ultrathin sections were obtained at 70-90nm on a Leica Ultracut UCT, and collected in a 200 mesh-grid. The sections were stained in uranyl acetate solution in ethanol and lead citrate, in order to be observed in a Phillips electron microscope Morgagni 268D.

Indirect Immunofluorescence. For indirect immunofluorescence, 3x105 cell/well (1ml) were plated in a 6-well culture dish. The cells were grown to 60-70% confluence. Then, 24 hours after confluence, the cells were rinsed twice in phosphate-buffered saline (PBS) for 5 minutes and fixed with 4% paraformaldehyde for 60 minutes. All cells were rinsed twice with tricine- buffered saline (TBS) for five minutes in order to eliminate any paraformaldehyde residues. Afterward, the cells were permeabilized with a 0.2% Triton X-100 in PBS. The cells were re-rinsed twice in TBS for five minutes and inespecific reactions were blocked with 3% BSA. The primary antibody incubation was carried out at 1:100 at 4ºC over night (Table 1). FITC-conjugated anti-goat was applied for Vimentin stained at 1:100 for 1h at room temperature. Similar procedure was performed using FITC-conjugated anti-mouse IgG (AP308F, Chemicon International, Temecula, CA, USA) for the other primary antibodies. The cells were rinsed twice with TBS for five minutes, followed by one wash with distillated water, mounted with Vectashield-DAPI (ABCYS, Paris, France) and examined with a LSM 510 (Carl Zeiss Microscopy, Jena, Germany).

RESULTS

Cell culture based on OE explants demonstrated rapid growth. Approximately 24 hours after plating the cells of olfactory biopsies, phase-bright spheres cells were found floating in culture flasks. In this phase, some cells were already adhering to the bottom of the culture flasks, though still surrounding the fragments (Fig.1a,b).




Culture medium was exchanged after a couple days. Clusters of the most viable cells were observed within the first week (Fig.1c). After 10 day of culture, these cells were collected from the monolayer after being rinsed twice in PBS, and dissociated in a 0.25% trypsin solution, following the seeding of 1x104 cells in a 25cm2 flask culture (Fig.1d). In the new flasks culture, proliferation, expansion and cell-clusters formations were also observed after trypsinization (Fig.1e,f).

At the beginning, a heterogeneous population was observed, although being homogeneous, and forming colonies of fusiform cells after 20 days, which fully expanded in the culture flask after two days (Fig.2a). For this culture, the medium was changed each four days, according to the confluence of cells in the flask, and maintaining the initial characteristic of the culture (Fig.2b).



Non-specific differentiation medium was used for developing the cell culture. However, from twentieth days, stellate cells resembling neuronal cells were observed (Figure 2c, d). Not so far, the stellate cells were also positive for neuronal immunostaining evidenced by GFAP-positive astrocytes expression (rhodamine-red staining), and nucleus in a central position stained with DAPI nuclear staining (Fig.3a,b).



In addition, immunostaining evidenced the presence of fusiform cells expressing positive labeling of neurofilaments (FITC-conjugated antibody), a specific component of the neuronal cytoskeleton (Fig.3c). In the same way, positive expression of other specific markers to neuronal progenitor such as oligodendrocyte and III â-tubulin was also identified (Fig.3d,e).

The Ki67 immunostaining showed a trend to label cells group throughout the apical region of the OE, with diffuse labeling near the basal lamina (Fig.4a). On the other hand, PCNA immunostaining label predominantly cells groups lying above the basal lamina (Fig.4b).



The transmission electron microscopy of OE from 60day aged dogs revealed cells with electron-dense cytoplasm and same distribution as those of cell staining positive for PCNA. Metabolic activity was confirmed by presence of euchromatin in the most of cells (Fig.5).


The respiratory epithelium was characterized as ciliated pseudostratified columnar epithelium due to the arrangement of the columnar epithelial cells. These cells presented cytoplasm with intermediary electron-density when compared with basal cells. Sustentacular cells were differentiated based on the absence of cilia and lower cytoplasmatic electron-density (Fig.6a). Olfactory neurons were visualized in close relationship with sustentacular cells. Neuronal metabolic activity was evidenced by the presence of numerous mitochondrias clustered near the nucleus (Fig.6b).


DISCUSSION

Culture of olfactory epithelium from 60-day aged dogs

Studies related to stem cells culture have been received special attention because stem cells demonstrate the capacity for renewal after trauma, also not only in basic neurogenic research, but also enabling the treatment of degenerative disease as neurological disorders, such as Parkinson's disease (Del Corral et al. 2003, Li et al. 2005, Zhang et al. 2006).

Stem cells culture from OE of experimental dog model (Krudewig et al. 2006, Overall et al. 2007) give subsidies to the establishment of protocols for obtaining progenitor cells committed with neuronal lineage of cells, avoiding to access the central nervous system.

Other author has reached promising outcomes based in dogs as an animal model used to evaluate diseases that can be find in human (Alves et al. 2009, Grando et al. 2009) or to obtain progenitor cells that can be applied in different types of cell therapy. In this way, Kerkis et al. (2008) transplanted a population of Human immature Dental Pulp Stem Cell into 4 littermate Golden Retriever Dogs affected by Muscular Dystrophy (GRMD), when these authors verified presence of significant engraftment in GRMD dog muscles with failure in the expression of dystrophin. These results support our data about the potential of dogs as an animal model in stem cell researches, and encourage the establishment of the canine model to compare with disease such as those seen in humans. Using this canine x-linked muscular dystrophy model, recent data presented controversies related to the real phenotypes variability presented by these dogs (Ambrósio et al. 2008, Ambrósio et al. 2009, Barthélémy et al. 2009) then pre-clinical results must be interpreted with care and attention.

Dog's OE explants maintained in culture in D-MEM/F12 for 60-day, demonstrated high rate of releasing cells in culture after 24 hours. Recent studies have demonstrated a remarkable functional plasticity in multilineage embryonic stem cells revealing high potential of differentiation, as well as an elevated mitogenesis (Lumelsky et al. 2001, Odorico et al. 2001). According to Pagano et al. (2000), this effect is related to its capacity of self-renewal and its unlimited potential for differentiation, when compared to adult cells. In their studies, stem cells isolated from the olfactory bulb and submitted to mitogenic growing factors constituted only one percent of true stem cells. The remaining cells were composed of the transient population, which eventually died or underwent differentiation.

Cells with high potential to confluence were observed attached to the flask at 5th day in culture. Similar observations were made by Murrell et al. (2005), when they established viable cells from 7 to 10 days in culture. In agreement, Krudewig et al. (2006) achieved total adhesion and confluence of cells isolated originated from olfactory bulb of dogs following 3 days in medium supplemented with forskoline and FGF-2. Particularly, in our culture, the complete confluence was only reached after 10 days.

After 20 days in culture, cells from OE were observed demonstrating fusiform morphology and maintaining high level of homogeneity. This characteristic was also reported by Pagano et al. (2000), Jin et al. (2002) and Zhang et al. (2005, 2006), when it was promoted differentiation of cells into the neuronal lineage through factor of neurogenic stimulation (EGF, FGF-2, and BDNF-brain-derived neurotrophic factor).

The fourth passage was characterized by the presence of stellate cells, evidencing cytoplasmic expansions which resemble the interaction observed among neuronal cells. This aspect was described by Roisen et al. (2001) during the eighteenth passage. Other authors as Krudewig et al. (2006), achieved same results in culture, among the sixth and ninth passages, and confirmed by immunostaining for GFAP and Fibronectin. However, the best results were obtained by Zhang et al. (2006), after treatment with RA1FNSShh and VAChT (Vesicular acetylcholine transporter), revealing neuritis formation and synaptic vesicles.

In our study, stem cells collected from OE of young dogs provided the opportunity of its future application in cell therapies. We detach that the cell culture protocol was based only in the isolation and expansion of cells without further differentiation induced-program. In addition, cell-to-cell interactions through cytoplasmatic projections and the tendency to form colonies supported the hypothesis of the potentiality of these cells to source neuronal lineages. A similar aspect was also observed by Calof et al. (2002) and Chandran et al. (2004) for GFAP- positive expression differentiated cells from human sub-ventricular zone and olfactory bulb.

The predominance of potential for growth and expansion in culture of cells from young dogs compared to adults produce cells whose morphology is similar to those reported in the literature as neuronal lineages.

PCNA and Ki67 immunostaining of cells from OE of 60-day aged

Immunostaining for proliferating cell nuclear antigen (PCNA) and Ki67 of the olfactory epithelium allowed to identify the most phases of the cell cycle as was described by Tsuji et al. (1992) and Pendleton et al. (1993) studying expression of protein markers in human.

High tendency for Ki67 expression was observed predominantly in the apical layer, when compared to PCNA immunostaining protocol whose showed positive labeling essentially above the basal layer, according to Aguiar (1996), Costa (1997), Bruck et al. (2001) in humans, and Alves et al. (2007) in dogs. Thus, although the Ki67 label most number of phases, all phases except Go (Capello et al. 2006), when compared with PCNA, it was able to identify allowed only measure the longest stages of this process (Jascur & Boland 2006), justifying the intensity of Ki67 labeling index present on the apical cells of OE, whose the division process occur more slowly.

The pseudostratified pattern of the OE from 60-day aged dog allowed labeling positive nuclear cells in different layer. This observation was supported by hypothesis that populations of stem cells are resident in middle and basal layer of the OE, as was described by Higuchi et al. (2005) studying dynamic of precursor of the OE in young Cavia sp. Similarly, Ohta et al. (2000) and Legrier et al. (2001) reached same results studying the cell cycle proliferation using PCNA technique as well as the presence of epidermal growth factor (EGFR) and neurogenic regulation in mices.

The ultrastructural analysis demonstrated morphological similarity between basal cells and those present in the middle layer and sustentacular epithelium as was described by Caggiano et al. (1994) and Huard et al. (1998). In addition, according to Nakamura et al. (1998) and Higuchi et al. (2005), sustentacular cells and olfactory neurons could be characterized by the presence of communicant gap junctions. Besides, numerous mitochondrias disperse evenly in the cytoplasm of neurons, as well as chromatin and euchromatin in the cytoplasm of basal cells.

CONCLUSION

These aspects give subsidies to support the hypothesis about resident progenitor cells among the basal cells of the OE, committed to generate all the constituents of this region, particularly sensorial neurons.

Acknowledgements.-To FAPESP (Fundação de Amparo à Pesquisa do Estado de São Paulo (Process Number 05/57787-6) and INCTC (Instituto Nacional de Ciências e Tecnologia em Céluas-tronco e Terapia Celular) for financial support.

Received on August 24, 2009. Accepted for publication on December 20, 2009.

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  • Publication Dates

    • Publication in this collection
      07 June 2010
    • Date of issue
      Apr 2010

    History

    • Accepted
      20 Dec 2009
    • Received
      24 Aug 2009
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