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Citation: Cell Death and Disease (2016) 7, e2217; doi:http://dx.doi.org/10.1038/cddis.2016.120

Web End =10.1038/cddis.2016.120

& 2016 Macmillan Publishers Limited All rights reserved 2041-4889/16 http://www.nature.com/cddis

Web End =www.nature.com/cddis

J Gao1,2, X-y Kang2, S Sun2, L Li2, B-l Zhang2, Y-q Li1 and D-s Gao*,1,2

Glial cell line-derived neurotrophic factor (GDNF) has strong neuroprotective and neurorestorative effects on dopaminergic (DA) neurons in the substantia nigra (SN); however, the underlying molecular mechanisms remain to be fully elucidated. In this study, we found that the expression level of transcription factor Six2 was increased in damaged DA neurons after GDNF rescue in vivo and in vitro. Knockdown of Six2 resulted in decreased cell viability and increased the apoptosis of damaged DA neurons after GDNF treatment in vitro. In contrast, Six2 overexpression increased cell viability and decreased cell apoptosis. Furthermore, genome-wide chromatin immunoprecipitation sequencing (ChIP-seq) indicated that Six2 directly bound to the promoter CAGCTG sequence of smad ubiquitylation regulatory factor 1 (Smurf1). ChIP-quantitative polymerase chain reaction (qPCR) analysis showed that Smurf1 expression was significantly upregulated after GDNF rescue. Moreover, knockdown of Six2 decreased Smurf1 expression, whereas overexpression of Six2 increased Smurf1 expression in damaged DA neurons after GDNF rescue. Meanwhile, knockdown and overexpression of Smurf1 increased and decreased p53 expression, respectively. Taken together, our results from in vitro and in vivo analysis indicate that Six2 mediates the protective effects of GDNF on damaged DA neurons by regulating Smurf1 expression, which could be useful in identifying potential drug targets for injured DA neurons.

Cell Death and Disease (2016) 7, e2217; doi:http://dx.doi.org/10.1038/cddis.2016.120

Web End =10.1038/cddis.2016.120 ; published online 5 May 2016

Neurotrophic factors have recently emerged as promising therapeutic drugs for neurodegenerative diseases. Among these, glial cell line-derived neurotrophic factor (GDNF) has attracted special attention for its protective effects on injured dopaminergic (DA) neurons in Parkinsons disease (PD).13 Although enhancing GDNF signalling protects damaged DA neurons, little is known about its protective mechanisms.

Apoptosis has been implicated as one of the important mechanisms leading to DA neuronal death in the substantia nigra (SN) of PD patients.4,5 Previous reports indicated that exogenous GDNF could improve the survival and reduce apoptosis of embryonic DA neurons.6,7 Similarly, the combined application of GDNF and caspase inhibitor enhances the survival of grafted DA neurons.8 In lactacystin-induced DA neurodegeneration, GDNF significantly inhibits DA neuron apoptosis and reduces caspase-3 activation.9 We previously demonstrated that GDNF protects 6-hydroxydopamine (6-OHDA)-injured MN9D cells by upregulating Bcl-2 and Bcl-w expression.10 Those studies suggested that an anti-apoptotic effect was likely the primary protective mechanism of GDNF on damaged DA neurons. However, the precise mechanisms remain to be fully elucidated.

Abbreviations: GDNF, Glial cell line-derived neurotrophic factor; DA neurons, dopaminergic neurons; PD, Parkinsons disease; SN, substantia nigra; 6-OHDA, 6-hydroxydopamine; SIX, sine oculis homeobox; Smurf1, smad ubiquitylation regulatory factor 1; CCK8 assay, cell counting kit-8 assay; QPCR, real-time polymerase chain reaction; ChIP, chromatin immunoprecipitation

Transcription factor Six2 mediates the protection of GDNF on 6-OHDA lesioned dopaminergic neurons by regulating Smurf1 expression

The transcription factor Six2 is a member of the sine oculis homeobox (SIX) family. It was previously identified as a critical regulator in normal kidney development.11,12 Several recent

lines of evidence have indicated that Six2 is also involved in organ development and some diseases.1315 Meanwhile, studies have also indicated that Six2 has the function of anti-apoptosis, for example, downregulated Six2 induces meta-nephric mesenchyme cell apoptosis,16 and miR181 could also promote apoptosis by targeting Six2 in vitro.17 We previously observed aberrant Six2 expression in damaged DA neurons after GDNF rescue, which led us to hypothesise that GDNF upregulates Six2 to prevent damaged DA neurons from undergoing apoptosis.

In the present study, we provide evidence that Six2 is pivotal for GDNF protection in injured DA neurons. Knockdown of Six2 by lentiviral shRNA and Six2 overexpression decreased and increased the protection afforded by GDNF, respectively. Further screening of Six2 targets by genome-wide chromatin immunoprecipitation sequencing (ChIP-seq) identified the smad ubiquitylation regulatory factor 1 (Smurf1) as a specific target of Six2, and this inhibited the apoptosis of damaged DA neurons. This study may be of significant value to identify potential drug targets for injured DA neurons.

1Department of Anatomy and Histology, The Fourth Military Medical University, Xian 710003, Shanxi, China and 2Department of Neurobiology and Anatomy, Xuzhou Key Laboratory of Neurobiology, Jiangsu Key Laboratory of New Drug Research and Clinical Pharmacy, Xuzhou Medical College, Xuzhou 221004, Jiangsu, China *Corresponding author: D-s Gao, Department of Neurobiology and Anatomy, Xuzhou Key Laboratory of Neurobiology, Jiangsu Key Laboratory of New Drug Research and Clinical Pharmacy, Xuzhou Medical College, 209 Tongshan Road, Xuzhou 221004, Jiangsu, China. Tel: +86 516 8326 2301; Fax: +86 516 8326 2301;

E-mail: mailto:[email protected]

Web End [email protected]

Received 26.10.15; revised 06.4.16; accepted 06.4.16; Edited by A Yaron

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Figure 1 Effects of GDNF on DA neurons in SN of PD rats. (A and B) Results of postural asymmetry and apomorphine-induced rotation of rats in all groups (16 g 6-OHDA for 2 w followed by different doses of GDNF for 1 w). Bar graphs are shown as means S.E.M. (n = 10). (C) Immunohistochemistry analysis of TH+ DA neuron after GDNF rescue in SN of PD rats (16 g 6-OHDA for 2 w followed by different doses of GDNF for 1 w). (a) Control group, (b) 6-OHDA group, (c) 6-OHDA+PBS group, (d) 6-OHDA+2 g GDNF group, (e) 6-OHDA+4 g GDNF group, (f) 6-OHDA+8 g GDNF group; scale bars (in af) equals 200 m. af are higher magnification images in af, scale bars equals 20 m. (D) Counting of the above TH+ DA neurons in the SN of PD rats after GDNF rescue. (E and F). TH mRNA and protein expression levels in damaged DA neurons after GDNF rescue in the SN of PD rats (16 g 6-OHDA for 2 w followed by different doses of GDNF for 1 d). Bar graphs are shown as means S.E.M. (n = 5). *Po0.05 versus control group, #Po0.05 versus the 6-OHDA group. The statistical analysis was carried out using one-way ANOVA followed by post hoc NewmanKeuls tests

Results

GDNF rescues 6-OHDA-damaged DA neurons. To verify that GDNF could protect damaged DA neurons, we generate a rat PD model using 6-OHDA. The posture asymmetry

experiment indicated that the frequency of head turning to the lesioned side improved after GDNF rescue (Figure 1A), in addition, apomorphine-induced rotation test confirmed that the motor abilities of PD rats were significantly improved, particularly in the 8 g GDNF groups (Figure 1B). To further

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Figure 2 Effects of GDNF on MES23.5 DA neurons in vitro. (a) Cell viability assay of MES23.5 DA neurons after 6-OHDA (100 mM) treatment of different time points. (b) Cell viability assay of MES23.5 DA neurons after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml) of different time points. (c) Cell counting with trypan blue staining after 6-OHDA (100 mM) treatment of different time points. (d) Cell counting with trypan blue staining after 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml) treatment of different time points. (e) Apoptosis rate analysis of MES23.5 DA neurons by flow cytometry after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (f) Expression of TH protein in DA neurons after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). *Po0.05 versus control group, **Po0.01 versus control group, #Po0.05 versus the 6-OHDA group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using one-way ANOVA followed by post hoc NewmanKeuls and post hoc Dunnetts tests

verify the protection of GDNF on damaged DA neurons, the numbers of TH+ DA neurons in the SN were counted. The numbers of TH+ neurons were significantly increased in the 8 g GDNF group compared with the 6-OHDA group; however, cell numbers were only slightly increased in the 4 g GDNF group and almost unchanged in the 2 g GDNF group (Figures 1Caf and D), indicating a dose-dependent effect. We also examined TH expression in the SN, and found that TH dose-dependently increased after GDNF rescue (Figures 1E and F). These results suggest that GDNF significantly protects damaged DA neurons in the SN of PD rats.

Moreover, we observed protective effects of GDNF on damaged MES23.5 DA cell line in vitro. The CCK8 assay results showed that cell viability decreased to approximately 50% after 6 h of 6-OHDA treatment and then increased after

12 h of GDNF rescue (Figures 2a and b). Similarly, cell counting with trypan blue staining and flow cytometry analyses both indicated that the cell apoptosis rate was about 50% at 6 h after 6-OHDA treatment and decreased after 12 h GDNF treatment (Figures 2c and d). The in vitro results (6-OHDA 6 h followed by GDNF 12 h) were similar with that for the in vivo experiments (6-OHDA 2 w followed by GDNF 1 w). Moreover, we also investigated that TH expression significantly increased after GDNF rescue in damaged MES23.5 DA neurons (Figure 2f). Collectively, these results suggest that GDNF efficiently protects DA neurons damaged by 6-OHDA in vivo and in vitro.

GDNF upregulates Six2 expression in 6-OHDA-damaged DA neurons. In order to detect whether Six2 expression was regulated by GDNF in damaged DA neurons, we assessed

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Figure 3 Six2 increased in damaged DA neurons after GDNF rescue in vivo and in vitro. (a and b) The mRNA and protein expressions of Six2 in the SN of PD rats in vivo models after GDNF rescue (16 g 6-OHDA for 2 w followed by different doses of GDNF for 1 d). (c and d) The mRNA and protein expressions of Six2 in damaged MES23.5 DA neuron models after GDNF rescue (100 mM 6-OHDA for 6 h followed by 100 ng/ml GDNF for 12 h). *Po0.05 versus control group, #Po0.05 versus the 6-OHDA group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using one-way ANOVA followed by post hoc NewmanKeuls tests. (e) The protein expressions of Six2 in the SN of PD rats in vivo models after GDNF treatment (8 g GDNF for 1 d). (f) The protein expressions of Six2 in cultured MES23.5 DA neurons after GDNF treatment (100 ng/ml GDNF for 12 h). *Po0.05 versus PBS group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using unpaired t-tests

Six2 mRNA and protein expressions in the SN of PD rats after GDNF rescue. Increased Six2 levels were highest in the 8 g GDNF group (Figures 3a and b). We also analysed Six2 expression changes in damaged MES23.5 DA neurons after GDNF rescue. The results revealed that Six2 was obviously increased (Figures 3c and d), which was consistent with the in vivo findings. We further detected whether GDNF could increase the Six2 protein level even without 6-OHDA challenge, the results indicated that the Six2 protein levels also increased after GDNF treatment both in vivo and in vitro (Figures 3e andf). Taken together, these results suggest that Six2 are involved in the GDNF-mediated protection of damaged DA neurons.

Six2 knockdown attenuates the protective effects of GDNF in damaged DA neurons. To test whether Six2 mediates the protection of GDNF in injured DA neurons, a lentivirus-mediated knockdown strategy was utilised to diminish Six2 expression. An shRNA (shSix2-2-pLV)

targeting Six2 decreased Six2 expression in MES23.5 DA neurons by approximately 90% (Figure 4a). We further found that the viability of cells infected with shSix2-pLV was reduced compared with pLV-infected MES23.5 DA neurons after GDNF rescue (Figure 4b). Cell counting with trypan blue staining showed that the dead rate of cells infected with shSix2-pLV was higher than that of control cells (Figure 4c). Similarly, flow cytometry analysis also showed that the apoptosis rate of cells infected with shSix2-pLV was higher than that of control cells (Figure 4d). In addition, the mRNA and protein expression levels of TH were also reduced in the shSix2-pLV group (Figures 4e and f). These results suggest that the transcription factor Six2 mediates the protective effects of GDNF on damaged DA neurons.

Six2 overexpression enhances the protective effects of GDNF in damaged DA neurons. To further demonstrate that Six2 mediates the protective effects of GDNF, we

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Figure 4 Knockdown of Six2 decreased the protective effects of GDNF on damaged DA neurons. (a) Identification of candidate shRNA-Six2 in MES23.5 DA neurons. (bd) Cell viability analysis, cell counting after trypan blue staining and flow cytometry apoptosis rate analysis in Six2-knockdown MES23.5 DA neurons after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (e and f) mRNA and protein expressions of TH in Six2-knockdown MES23.5 DA neurons after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). *Po0.05 versus control group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using one-way ANOVA followed by post hoc NewmanKeuls tests

generated stably Six2 overexpression MES23.5 cells. Real-time PCR and western blot analysis demonstrated that Six2 was obviously increased in the Six2 overexpression group (Figures 5A and B). Importantly, damaged MES23.5 cell viability increased after GDNF rescue in the Six2 overexpression group compared with the control group (Figure 5C). Cell counting with trypan blue staining indicated that the dead rate of cells infected Six2-pLV was lower than that of control cells (Figure 5D). In accordance with the above findings, flow cytometry analyses indicated that the apoptosis rate of cells infected Six2-pLV decreased than that of control cells (Figure 5E). In addition, TH expression was significantly increased (Figures 5F and G). We further detected whether Six2 overexpression alone could reduce 6-OHDA toxicity in the absence of GDNF, results showed that MES23.5 cell viability increased in the Six2 overexpression group compared with the control group (Figure 5H), the dead rate of cells decreased in Six2 overexpression group (Figure 5I), and the apoptosis rate of cells also decreased in Six2 overexpression group (Figure 5J). In addition, the in vivo

experiments indicated that the numbers of TH+ neurons were significantly increased in the Six2 overexpression group in SN of PD rats (Figures 5K and L). Thus, our findings strongly indicate that Six2 is involved in the protective effects of GDNF on DA neurons.

Six2 mediates GDNF protection by upregulating Smurf1 expression. Our results clearly demonstrate that Six2 is critical for regulating GDNF protection. For an unbiased assessment of the plausible mechanisms of Six2, we performed a genome-wide ChIP-seq analysis for Six2 in MES23.5 DA neurons. The peaks of Six2 occupancy were often broad, with some around 1 kb (Figure 6a). We successfully detected 384 differential genes between DA neurons treated with 6-OHDA followed by GDNF group and DA neurons treated with 6-OHDA group (Supplementary Table 1). Of the Six2-binding sites, 7.2% were located in the region of 2000 bp upstream from transcription start site of the 384 differential genes (Figure 6b). We also performed de novo motif discovery to identify specific sequences bound

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by Six2 (Figure 6c), among these differentially expressed genes, Six2 directly bound to the promoter CAGCTG sequence of smad ubiquitylation regulatory factor 1 (Smurf1). Smurf1 was significantly upregulated after GDNF rescue by ChIP-qPCR analysis (Figure 6d), the protein expression of Smurf1 also increased after GDNF rescue both in vivo and in vitro by western blot analysis (Figures 6e and f). We further

found that Smurf1 expression decreased in cells infected with shSix2-pLV and increased in Six2 overexpression cells after GDNF rescue (Figures 6g and h). We also found that Smurf1 overexpression in 6-OHDA- and GDNF-treated MES23.5 cells with downregulated Six2 could increase cell viability by CCK8 analysis (Figure 7A), decrease the dead rate of cells by cell counting with trypan blue staining (Figure 7B)

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and decrease the apoptosis rate of cells by flow cytometry analyses (Figure 7C). In addition, we further detected whether Smurf1 overexpression alone could reduce 6-OHDA toxicity in the absence of GDNF, results showed that MES23.5 cell viability increased in the Smurf1 overexpression group (Figure 7D), the dead rate of cells decreased in Smurf1 overexpression group (Figure 7E) and the apoptosis rate of cells also decreased in Smurf1 overexpression group (Figure 7F). In addition, the in vivo experiments indicated that the numbers of TH+ neurons were significantly increased in the Smurf1 overexpression group in SN of PD rats (Figures 7G and H). These results suggest that Six2 mediates the protective effects of GDNF on damaged DA neurons by upregulating Smurf1.

Smurf1 mediates GDNF protection by degrading p53. Previous study showed that Smurf1 could promote the degradation of p53.18 We first detected the protein expression of p53 after GDNF rescue, the results showed that the p53 protein levels decreased after GDNF rescue in SN of PD rats (Figure 8a). To further test whether Smurf1 mediates the protection of GDNF by degrading p53 in injured DA neurons, a Smurf1 shRNA plasmid (shSmurf1-plasmid) decreased Smurf1 expression in MES23.5 cells by approximately 50%. We further found that the protein expression levels of p53 were increased in the shSmurf1-plasmid group after GDNF rescue (Figure 8b). In addition, we also generated stably Smurf1 overexpression MES23.5 cells. Western blot analysis demonstrated that p53 obviously reduced in the Smurf1 overexpression (Smurf1-pLV) group after GDNF rescue (Figure 8c). These results suggest that the Smurf1 mediates the protective effects of GDNF on damaged DA neurons by degrading the p53 expression.

Six2 knockdown and overexpression attenuates and increases the protective effects of GDNF in SN of PD rats, respectively. To further demonstrate whether Six2 mediates the protective effects of GDNF on PD rats, we injected shSix2-pLV or Six2-pLV encoded EGFP into SN of PD rats, and then investigated the motor ability after GDNF rescue. Immunofluorescence staining analysis showed these viral-encoded EGFP was, respectively, expressed in TH+ neurons in SN of PD rats after GDNF rescue (Figure 9A). Western blot analyses demonstrated that Six2 was obviously decreased in the Six2 knockdown group and increased in the Six2 overexpression group, while GDNF expression were

consistent among different groups in SN of PD rats after GDNF rescue (Figures 9B and C). The numbers of TH+ neurons were significantly increased in the Six2 overexpression group, and decreased in the Six2 knockdown group in SN of PD rats after GDNF rescue (Figures 9D and E). The posture asymmetry experiment indicated that the frequency of head turning into the lesioned side decreased after Six2 knockdown, and apomorphine-induced rotation increased after Six2 knockdown (Figures 9F and G). Although over-expression of Six2 could promote a little motor ability, but there was no statistical significance (Figures 9H and I). These results indicated that Six2 is involved in the protective effects of GDNF on PD rat models.

Discussion

GDNF has been shown to ameliorate neurodegeneration in neurotoxin-induced rats and nonhuman primate models of PD;1921 however, the underlying molecular mechanisms remain largely unknown. Our results are the first evidence that Six2 is at least partially responsible for the protective effects of GDNF in damaged DA neurons. Furthermore, we showed that Smurf1 was directly regulated by Six2 after GDNF rescue, and this inhibited the apoptosis of damaged DA neurons.

GDNF has strong protective effects on DA neurons in the SN of PD models. Previous reports showed that injection of single high doses of GDNF 1 or 3 months after the toxic insult induced upregulation of TH expression and promoted the motor ability of PD models obviously.22,23 Our findings

provided additional evidence that single doses of GDNF 2 weeks after 6-OHDA lesion rescued the damaged DA neurons and improved the motor ability of PD rats. This hypothesis is reinforced by the fact that GDNF has been shown to reverse toxin-induced injury to DA neurons.24,25 In

this study, we also showed the TH mRNA and protein expression increased 1 day after GDNF injection. A previous study showed that injection of 125I-labelled GDNF into striatum, the obvious fluorescence in SN could be detected 6 h after injection, and lasted for several days.26 Long-time surveillance showed that the numbers of TH+ DA neurons increased from 2 to 21 days in cultured rat embryo midbrain cells treated with GDNF than in control groups.2 In addition, the motor activity of rats increased from 2 to 10 days after GDNF injection, the apomorphine-induced rotation behaviour increased most obviously 1 week after GDNF injection.25,27

Figure 5 Overexpression of Six2 increased the protective effects of GDNF on damaged DA neurons. (A and B) The mRNA and protein expressions of Six2 in Six2-overexpressed MES23.5 DA neuron models. (CE) Cell viability, cell counting after trypan blue staining and flow cytometry apoptosis rate analysis of Six2-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (F) Expression of TH mRNA in Six2-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (G) Expression and quantification of TH protein in Six2-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). *Po0.05 versus control group, **Po0.01 versus control group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using one-way ANOVA followed by post hoc Dunnetts tests. (H) Cell viability analysis of Six2-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h). (I) Cell counting after trypan blue staining analysis of Six2-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h). (J) Flow cytometry apoptosis rate analysis of Six2-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h). (K) Immunohistochemistry analysis of TH+ DA neuron after Six2 overexpression in SN of PD rats in vivo models (16 g 6-OHDA for 2 w). (a) pLV group,(b) Six2-pLV group; scale bars (in a and b) equals 200 m. a and b are higher magnification images in a-b, scale bars equals 20 m. (L). Counting of the above TH+ DA neurons in the SN of PD rats in vivo models after Six2 overexpression. * Po0.05 versus pLV group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using unpaired t-tests

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According to the above studies, we detected the TH mRNA and protein expression after 1 day of GDNF injection, and detected the numbers of TH+ DA neurons and behavioural

tests after 1 week of GDNF injection in this study. These findings provided additional evidence that GDNF has strong protective effects on damaged DA neurons.

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Figure 7 Smurf1 overexpression could rescue the injured DA neurons. (A) Cell viability analysis of Smurf1-overexpressed MES23.5 DA neuron models with downregulated Six2 after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (B) Cell counting after trypan blue staining of Smurf1-overexpressed MES23.5 DA neuron models with downregulated Six2 after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (C) Flow cytometry apoptosis rate analysis of Smurf1-overexpressed MES23.5 DA neuron models with downregulated Six2 after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). *Po0.05 versus shSix2-pLV group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using unpaired t- tests. (D) Cell viability analysis of Smurf1-overexpressed

MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h). (E) Cell counting after trypan blue staining analysis of Smurf1-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h). (F) Flow cytometry apoptosis rate analysis of Smurf1-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h). (G) Immunohistochemistry analysis of TH+ DA neuron after Smurf1 overexpression in SN of PD rats in vivo models (16 g 6-OHDA for 2 w). (a) pLV group, (b) Smurf1-pLV group; scale bars (in a and b) equals 200 m. a and b are higher magnification images in a and b, scale bars equals 20m. (H) Counting of the above TH+ DA neurons in the SN of PD rats in vivo models after Smurf1 overexpression. *Po0.05 versus pLV group. Bar graphs are shown as means S.E.M. (n = 3). The statistical analysis was carried out using unpaired t-tests

Figure 6 Six2 mediated the protection of GDNF on DA neurons by upregulating Smurf1 expression. (a) Peaks of Six2 occupancy in genomic fragments in MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (b) Loci distribution of Six2-bound differential expressed target genes in MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). The word 'down2k' means 2000 bp downstream from the transcription termination site of the genes, 'up2k' means 2000 bp upstream from the transcription start site of the genes, 'exon' means exon region of the genes, 'intron' means intron region of the genes. (c) Potential candidate motifs prediction of Six2 in MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (d) Chromatin immunoprecipitation assay with anti-Six2 antibody for Smurf1 in MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h), ChIP DNA was quantified by qPCR and normalised to input. (e) The protein expression and quantitative analysis of Smurf1 in MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (f) The protein expression and quantitative analysis of Smurf1 in the SN of PD rats in vivo models after GDNF rescue (16 g 6-OHDA for 2 w followed by 100 ng/ml GDNF for 1 d). (g) Expression and quantification of Smurf1 protein in Six2-knockdown MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (h) Expression and quantification of Smurf1 protein in Six2-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). *Po0.05 versus the control group, #Po0.05 versus the 6-OHDA group. Bar graphs are shown as means S.E.M.

(n = 3). The statistical analysis was carried out using t-test and one-way ANOVA followed by post hoc NewmanKeuls tests and post hoc Dunnetts tests

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The transcription factor Six2 has been suggested to be involved in kidney development,13,28 and Six2 downregulation

results in renal mesenchymal stem cell apoptosis.16 Our

in vivo and in vitro analysis showed that Six2 mRNA and protein expression was upregulated in damaged DA neurons after GDNF rescue. These results imply that Six2 mediates GDNF protection. Indeed, knockdown and overexpression experiments in vitro confirmed that Six2 mediates the protective anti-apoptotic effect of GDNF, and our in vivo analysis also demonstrated that Six2 could protect damaged

DA neurons and improve the motor ability of PD rats. Other studies showed that Six1, another member of the SIX family, played critical roles in protecting neurons from apoptosis.2931

Six1 may also have potential protective functions in DA neurons similar to Six2 because of its similar conserved sequence. Now, the related experiments about Six1 are under way in our laboratory and we wish it would be finished as quickly as possible.

Cell apoptosis occurs via the activation or inhibition of apoptosis-associated factors. Several factors including caspases, p53, and the ubiquitin proteasome system

Figure 8 Smurf1 mediated the protection of GDNF on DA neurons by degrading p53. (a) The protein expression and quantitative analysis of p53 in the SN of PD rats in vivo models after GDNF rescue (16 g 6-OHDA for 2 w followed by 8 g GDNF for 1 d). (b) The protein expression and quantitative analysis of Smurf1 and p53 in Smurf1-knockdown MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). (c) Expression and quantification of Smurf1 and p53 protein in Smurf1-overexpressed MES23.5 DA neuron models after treatment with 6-OHDA (100 mM, 6 h) followed by GDNF (100 ng/ml, 12 h). The data were from at least three independent experiments in each case. *Po0.05 versus control group of Smurf1, #Po0.05 versus control group of p53. Bar graphs are shown as means S.E.M. The statistical analysis was carried out using one-way ANOVA followed by post hoc Dunnetts tests

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modulate cell apoptosis in damaged DA neurons.5,3234

A previous study showed that overexpression of dominant-negative mutants of caspase-3, -7, and -9 could block the death of embryonic DA neurons induced by deprivation of GDNF.35 Other studies showed that GDNF/RET signalling were required for normal mitochondrial function and morphology, and blocking caspase-6 could inhibit the death of GDNF-deprived DA neurons.36,37 In addition, overexpression of Nurr1 could reverse the blockade of GDNF signalling, which was induced by deprivation of -synuclein in SN DA neurons.38 In

this study, although we have shown that Six2 could mediate the protective anti-apoptotic effect of GDNF, the factors that are directly modulated by Six2 after GDNF rescue have not been identified. In this study, ChIP-seq enabled us to investigate the underlying molecular mechanisms governing Six2-mediated protection by GDNF in damaged DA neurons at the genome level. Our results indicated that Smurf1 was targeted by Six2. Smurf1 belongs to the Nedd4 (neuronal precursor cell-expressed developmentally downregulated 4) family of HECT-type E3 ligases and has critical roles in regulating cell growth, migration, and autophagy.39 A previous study showed that Smurf1 could promote the degradation of p53,18 which is one of the key effectors promoting apoptosis.40,41 In this study, our results also indicated that

p53 was degraded by Smurf1 in damaged DA neurons after GDNF treatment. Our results provided additional evidence that the apoptosis of damaged DA neurons could be rescued by GDNF. Taken together, these findings demonstrate that the Six2 is a critical factor that mediates GDNF protection of damaged DA neurons by directly activating Smurf1, which could further degrade p53.

In summary, our results demonstrate that Six2 is a critical regulator of GDNFs ability to inhibit apoptosis of damaged DA neurons by upregulating the expression of Smurf1, which could further degrade p53. These findings provide new important evidence for the protective mechanism of GDNF, which could be useful in identifying potential drug targets for injured DA neurons.

Materials and MethodsAnimals and cell culture. Adult male (230250 g) Sprague Dawley rats were provided by Xuzhou Medical College. They were housed under controlled conditions (temperature 23 2 C and illumination 12:12 h lightdark cycle) with standard diet and water ad libitum. Animal housing and treatment of the rats were performed in accordance with the Guidelines of the Ethical Committee for Use of Laboratory Animals.

MES23.5 DA neurons and 293T cells were obtained from the Shanghai Institutes for Cell Resource Center at the Chinese Academy of Sciences (Shanghai, China). All cell lines were cultured in Dulbeccos modified Eagles medium, supplemented with 10% foetal bovine serum (Hyclone, Logan, UT, USA), 100 units/ml penicillin, and0.1 mg/ml streptomycin (Invitrogen, Carlsbad, CA, USA) in a 5% CO2 atmosphere at 37 C.

Reagents and antibodies. The 6-OHDA (H116) and GDNF (G1401) were purchased from Sigma (St. Louis, MO, USA). Rabbit anti-Six2 (SAB2103006), rabbit anti-GDNF antibody (SAB1401150), mouse anti-tyrosine hydroxylase (TH) (T2928), and rabbit anti-Smurf1 antibody (S8449) were also from Sigma. The rabbit anti-Six2 antibody (sc-135274) was from Santa Cruz (St. Louis, MO, USA).The rabbit anti-p53 antibody (BS3736) was from Bioworld Technology (Shanghai, China). The plasmid mini kit (74104) and midi kit (12143) were from Qiagen (Venlo, The Netherlands).

Constructing of PD rat models using 6-OHDA. The Sprague Dawley rats were anaesthetised with intraperitoneal sodium pentobarbital (50 mg/kg) and placed in the stereotaxic apparatus (bite bar at 3.3 mm). Damage was induced by unilateral stereotaxic injections of 6-OHDA (16 g total, 4 g/l with 2 l per site)

into the left striatum at two coordinates: (i) 0.7 mm anterior and 3 mm lateral to the bregma and 7 mm ventral to the cranial surface and (ii) 0.7 mm anterior and 3 mm lateral to bregma and 5 mm ventral to the cranial surface. The sham-operated rats received injections containing vehicle (0.1% ascorbate in 0.9% saline) at the same coordinates. All injections were performed using a 26-gauge Hamilton syringe connected to an infusion minipump (Hamilton Co., Reno, NV, USA), at a rate of 1 l/min. After the injection, the syringe was left in place for 5 min and slowly retracted. Two weeks after 6-OHDA injection, the PD rats were screened using behavioural tests. Then, the GDNF was injected into the left striatum of the PD rat models.

Injection of GDNF into left striatum of PD rat models. This experiment was divided into six groups: (i) Control group: the normal rats (n = 20);(ii) 6-OHDA group: the rats received left striatum injection of 6-OHDA (n = 20);(iii) 6-OHDA+ phosphate buffered saline (PBS) group: the PD rats received left striatum injection of PBS (n = 20); (iv) 6-OHDA+2 g GDNF: the PD rats received left striatum injection of 2 g GDNF (n = 20); (v) 6-OHDA+4 g GDNF: the PD rats received left striatum injection of 4 g GDNF (n = 20); (vi) 6-OHDA+8 g GDNF: the PD rats received left striatum injection of 8 g GDNF (n = 20). One day after GDNF injection, 5 rats in every group were killed and the left sides of SN were processed for real-time polymerase chain reaction (qPCR) analysis, and 5 rats in every group were killed and the left sides of SN were processed for western blot analyses. One week after GDNF injection, the other 10 rats in every group were subjected to behavioural tests, and then, these rats were anaesthetised with sodium pentobarbital and transcardially perfused for immunohistochemistry analyses.

Behavioural analysis. The following behavioural tests were carried out 2 weeks after 6-OHDA injection for screening the PD rats, and 1 week after GDNF injection for detecting the effect of GDNF on PD rats.

Postural asymmetry: Postural asymmetry was analysed using the elevated body swing test as described previously.42,43 The rats were examined for lateral

movements with their bodies suspended by their tail 10 cm above the testing table. The frequency of head turning contralateral to the lesioned side (ipsilateral side) was evaluated in 20 continuous trials. Computing method was: (contralateral turns ipsilateral turns)/total turns 100%.

Apomorphine-induced rotation analysis: Contralateral rotations of each rat were recorded after subcutaneously injection of apomorphine (0.5 mg/kg in normal saline containing 0.01% ascorbic acid) to confirm the dopamine depletion in nigrostriatal system. The rotation behaviour was counted over a period of 60 min. The results were expressed in rotations/30 min.

Immunohistochemistry. As described previously,43 after behavioural tests, 10 rats in every group were anaesthetised and perfused through the left ventricle via an ascending aortic cannulation. According to Paxinos & Watsons The Rat Brain in Stereotaxic Coordinates, we used a stereotaxic apparatus to identify the brain segments containing the SN, which were consecutively sectioned on a microtome in the coronal plane at 6 m thickness. After blocking for nonspecific binding with 10% donkey serum albumin, these sections were incubated, respectively, with anti-TH antibody and biotinylated horse anti-mouse IgG, followed by the Elite avidin-biotin complex. The reaction was completed with 3'-diaminobenzidine, nickel II sulphate, and H2O2. Then,

these sections were mounted on gelatin-coated slides, dehydrated through graded alcohol, cleared in xylene, and cover-slipped with cytoseal for cell counting.

Stereology. The numbers of TH+ DA neurons in the SNpc (4.7 to 6.3 mm from bregma) on the injured side were counted under a light microscope.44 The first

sampling item was taken at random from the frontal part of the SNpc, every sixth section (6 m thickness) was selected. Sampling was carried out using the Olympus C.A.S.T.-Grid system (Olympus Albertslund, Denmark A/S, Denmark). The SNpc was carefully outlined to exclude other subdivisions of the substantia nigra and the ventral tegmental area by using a 4 objective. The total number of TH+ neurons was analysed using a 100 Planapo oil immersion objective with a 1.4 numerical aperture. Counting frame (60 um 60 um) was superimposed on the

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image of tissue sections. TH+ neurons were counted only when present completely or partially inside the frame and when they did not touch any of the red exclusion lines, neurons which touched green inclusion lines were counted. Neurons counted in all sections of the SNpc were summed to give a total number of TH+ neurons.

MES23.5 DA neurons treated with 6-OHDA and GDNF. The MES23.5 cell lines treated with 6-OHDA (100 mM) for different times (30 min, 1 h, 3 h, 6 h, 12 h, and 24 h) were selected for cell counting kit-8 assay (CCK8), trypan blue staining cell viability assay, real-time PCR, and western blot analysis.

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The MES23.5 DA neurons treated with 6-OHDA (100 mM) for 6 h followed by GDNF (100 ng/ml) for different times (0 h, 3 h, 6 h, 12 h, and 24 h) were also selected for CCK8 assays, cell counting with trypan blue staining, real-time PCR, and western blot analysis.

Real-time PCR analysis. Total RNA from the tissue samples and cell lines was extracted using high pure RNA isolation kits (Roche Applied Science, Indianapolis, IN, USA). RNA concentration and quality were determined with a Nanodrop ND-1000 spectrophotometer (NanoDrop Technologies, Wilmington, DE, USA) and gel analysis. Then, the RNA was reversely transcribed to cDNA using transcriptor first strand cDNA synthesis kit (Roche Applied Science). The expression of Six2 and TH genes was assayed using the SYBR green PCR master mix (Roche Applied Science). The mRNA data were normalised to -actin. The primers for Six2, TH, and -actin were as follows:

Six2-forward, 5- GAGGAGACCAGCTACTGCTTCAA-3, Six2-reverse, 5- TTGTGGCTACTGGAATTGGAGTTCT-3;

TH-forward, 5- TCTATGCTACCCATGCCTGCC-3, TH-reverse, 5- AAATCACGGGCGGACAGTAGAC-3;

-actin-forward, 5- CACCCGCGAGTACAACCTTC-3, -actin-reverse, 5- CCCATACCCACCATCACACC-3.

Western blot analysis. As described previously,45 total protein from the tissue samples and cell lines was extracted. Equal amounts of protein samples were separated by sodium dodecyl sulphate/polyacrylamide gel electrophoresis and then transferred onto nitrocellulose membranes (Amersham Pharmacia Biotech, Little Chalfont, UK). After blocking with 3% (w/v) bovine serum albumin for 3 h, the membranes were incubated with primary antibodies and then probed with goat anti-rabbit IR-Dye 670 or 800 cw-labelled secondary antibody. Membranes were imaged using a LiCor Odyssey scanner (Pleasanton, CA, USA). The western blot data were normalised to -actin.

Establishment of the MES23.5 DA neurons stably expressing shRNA-Six2. Five different targeted sequences homologous to Six2 were designed using the lentiviral expression vector (pLV-H1-EF1a-Bsd). Target sites were as follows: shSix2-1 sense strand, 5-CCAAGGAAAGGGAGAACAA-3;

shSix2-2 sense strand, 5-GCTACTGCTTCAAGGAAAA-3; shSix2-3 sense strand, 5-AGAATGAAAGCGTGCTCA-3; shSix2-4 sense strand, 5-CAGCCAACCTCGTG

GACCT-3; and shSix2-5 sense strand, 5-GCAACTTCCGCGAGCTCTA-3. These plasmid DNAs transcribed shRNA with loop sequences of 5-CTTCCTGTCAGA-3.

The negative control sequence was shScramble sense strand, 5-GACTTCATA GGCGCATGC-3. The constructed vector plasmid was transfected into 293T cells together with the packaging plasmids using Lipofectamine 2000 (Invitrogen);

the supernatants were collected after 48 h for virus purification. The purified virus containing shSix2-pLV was transfected into MES23.5 cells. After 96 h, cells were passaged and cultured using medium containing puromycin at a final concentration of 2 g/l. After seven passages when there was almost no cell death, the MES23.5 cell line stably expressing shRNA-Six2 was established. The cells were harvested for western blot to confirm Six2 knockdown. The cell lines with high knockdown efficiency were treated with 6-OHDA (100 mM) for 6 h followed by GDNF (100 ng/ml) for 12 h, and then selected for CCK8 assays, cell counting with trypan blue staining, flow cytometry analysis, real-time PCR, and western blot analysis.

Establishment of the MES23.5 DA neurons stably expressing Six2 (or Smurf1). MES23.5 cells were harvested to extract total RNA. Reverse

transcription and amplification of Six2 (or Smurf1) were carried out using Six2 (or Smurf1) upstream and downstream primers, and we then constructed a lentiviral expression vector (pLV-H1-EF1a-Bsd). After sequencing, purified plasmids without mutations and deletions were transfected into 293T cells together with packaging plasmids, as described above. The general protocols included transfecting MES23.5 cells using purified virus and selecting MES23.5 stably expressing Six2 (or Smurf1) using medium containing puromycin. The stably transfected MES23.5 cells were treated with 6-OHDA (100 mM) for 6 h followed by GDNF (100 ng/ml) for 12 h and analysed. The primers of Six2 and Smurf1 were as follows:

Six2: forward, 5-GCGGAATTCATGTCCATGCTGCCCACCTTC-3; reverse, 5-GCGGTCGACGGAGCCCAGGTCCACGAGGTT-3.

Smurf1: forward, 5-GCGGAATTCATGTCGAACCCCGGGACCCG-3; reverse, 5-GCGGTCGACTCACTCCACGGCAAAGCCACA-3.

Smurf1 shRNA plasmids transfection. Smurf1 shRNA plasmid (sc-41674-SH) was from Santa Cruz Biotechnology (Santa Cruz de la Sierra, Bolivia), this plasmid was transfected into MES23.5 cells using lipofectamine 2000 (Invitrogen). Forty-eight hours after transfection, the transfected cells were treated with 6-OHDA (100 mM) for 6 h followed by GDNF (100 ng/ml) for 12 h, and the samples were harvested for western blot analysis.

Cell viability assay. Cell viability assay was performed using a cell counting kit-8 assay (CCK8; Dojindo Laboratories, Shanghai, China) and a trypan blue staining cell viability assay kit (Beyotime, Jiangsu, China).

Evaluation of cell apoptosis by flow cytometry analysis. Cells were harvested using 0.25% trypsin and then washed with 0.1 M PBS. After centrifugation at 800 g for 5 min, cells were treated with 100 l binding buffer and then stained with 2 l propidium iodide and 2 l annexin V-fluorescein isothiocyanate for 15 min. In this study, an annexin-V-FLUOS staining kit (Roche Applied Science) was used to assess cell apoptosis, we used the BD FACSCalibur flow cytometry (Becton, Dickinson and Company, Franklin Lakes, NJ, USA) and the MACSQuant flow cytometry (Miltenyi Biotechnology, Bergisch Gladbach, Germany) to examine the cell apoptosis.

ChIP-seq and ChIP-qPCR. MES23.5 DA neurons were treated with 6-OHDA (100 mM) for 6 h followed by GDNF (100 ng/ml) for 12 h; 12 h after GDNF treatment, cells were fixed in 1% formaldehyde for 10 min, followed by quenching with glycine and rinsing with cold PBS. Afterwards, cells were collected and lysed. The nuclei were released and sonicated into 200700-base pair (bp) DNA fragments. Aliquots of chromatin were incubated overnight with 5 mg anti-Six2 antibody or control rabbit immunoglobulin G (rIgG, sc-2027) (Santa Cruz Biotechnology, Santa Cruz, CA, USA). The chromatin-antibody complexes were pulled down with prewashed Dyna beads (Invitrogen), washed, and eluted. DNA fragments associated with Six2 or control antibodies were eluted and purified. Input genomic DNA was obtained through similar elution and purification procedures. Prepared DNA was processed for ChIP-seq or ChIP-qPCR. The data from ChIP-seq were analysed by Motif analysis. Real-time qPCRs were performed with the primer pairs as follows:

Smurf1: forward, 5-CTCACTGGCATAGGGTTCCT-3; reverse, 5-TACAGGTGTGCTGGTGAGTT-3.

Substantia nigra lentivirus infection to measure Six2 expression and the motor ability of PD rats after GDNF treatment. The adult adult male (230250 g) Sprague Dawley rats were randomly divided into three

Figure 9 Six2 knockdown and overexpression attenuates and increases the protective effects of GDNF in SN of PD rats, respectively. (A) Immunofluorescence staining analysis showed the co-localisation of EGFP and TH in DA neurons in SN of PD rats after GDNF rescue (16 g 6-OHDA for 2 w followed by 8 g GDNF for 1 w) (red: TH; green: pLV, Six2-pLV and shSix2-pLV, respectively; blue: DAPI). Scale bars: 100 m. (B) Expression and quantification of Six2 and GDNF in SN of PD rats infected with shSix2-pLV after GDNF rescue (16 g 6-OHDA for 2 w followed by 8 g GDNF for 1 d). (C) Expression and quantification of Six2 and GDNF in SN of PD rats infected with Six2-pLV after GDNF rescue (16 g 6-OHDA for 2 w followed by 8 g GDNF for 1 d). (D) Immunohistochemistry analysis of TH+ DA neuron after GDNF rescue in Six2 overexpression group in SN of PD rats (16 g 6-OHDA for 2 w followed by 8 g GDNF for 1 w). (a) pLV group, (b) shSix2-pLV group, (c) Six2-pLV group; scale bars (in ac) equals 200 m. ac are higher magnification images in a and b, scale bars equals 20 m. (E) Counting of the above TH+ DA neurons in the SN of PD rats after GDNFrescue. (F and G) Postural asymmetry tests and apomorphine-induced rotation tests in PD rats infected with shSix2-pLV after GDNF rescue (16 g 6-OHDA for 2 w followed by 8 g GDNF for 1 w). (H and I) Postural asymmetry tests and apomorphine-induced rotation tests in PD rats infected with Six2-pLV after GDNF rescue (16 g 6-OHDA for 2 w followed by 8 g GDNF for 1 w). *Po0.05 versus control or pLV group. Bar graphs are shown as means S.E.M. (n = 8). The statistical analysis was carried out using one-way ANOVA followed by post hoc Dunnetts tests

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groups: (i) pLV groups (n = 11), in which the rats received a left substantia nigra injection of pLV-EGFP and left striatum injection of 6-OHDA followed by 8 g GDNF;(ii) Six2-pLV groups (n = 11), in which the rats received a left substantia nigra injection of Six2-pLV-EGFP and left striatum injection of 6-OHDA followed by 8 g GDNF; (iii) shSix2-pLV groups (n = 11), in which the rats received a left substantia nigra injection of shSix2-pLV-EGFP and left striatum injection of 6-OHDA followed by 8 g GDNF.

The rats were anesthetized with chloralic hydras (10%) and placed in a stereotaxic frame. Burr holes were drilled to permit unilateral stereotaxic injection of 4 l Six2-pLV or shSix2-pLV or pLV (the final title was 6 107 infectious units/ml) at a rate of 1 l/min into the left SN (stereotaxic coordinated from bregma: anteroposterior: 5.3 mm from bregma, mediolateral: 2.3 mm, and dorso-ventral: 8.3 mm below the surface of the dura). The 6-OHDA lesions were induced as above (see Materials and Methods:

Constructing of PD rat models using 6-OHDA), which was injected immediately following substantia nigra pLV delivery. Two weeks after 6-OHDA injection, the apomorphine-induced rotation analysis was used to screen the PD rat models.

Then, GDNF was injected into these PD rats (see Materials and Methods: 2.4 GDNF treatment), 1 day after GDNF treatment, the SN of three rats in every group were quickly removed into liquid nitrogen and used for western blot analysis of Six2 expression. One week after GDNF treatment, the other eight rats in each group were subjected to behavioural tests. After behavioural tests, these rats were deeply anesthetized and perfused, sections were made and collected as described above. These sections were incubated with anti-TH antibody and then with the secondary antibodies. Images were captured with a confocal laser scanning microscope (TCS SP2; Leica, Wetzlar, Germany). For display, images were merged and processed with Leica confocal software (TCS SP2 version 2.5). Only minor adjustments of brightness and contrast were made to the entire images.

Statistical analysis. All data were processed with SPSS 13.0 (SPSS Inc., Chicago, IL, USA). Bar graphs are shown as means S.E.M. Difference was carried out using t test to compare two independent samples, and one-way analyses of variance (ANOVAs) followed by post hoc NewmanKeuls tests to compare all pairs of groups or post hoc Dunnetts tests for comparing all experimental groups with the control group. Po0.05 was considered statistically significant for all tests.

Conflict of InterestThe authors declare no conflict of interest.

Acknowledgements. This project was supported by the National Natural Science Foundation of China (Grant numbers 31040035 and 81401056), Natural Science Foundation of Jiangsu Province (BK20130212), China Postdoctoral Science Foundation funded project (2013M540566), and a project funded by the Priority Academic Program Development (PAPD) of Jiangsu Higher Education Institutions.

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