Aging is the greatest risk factor for the development of Parkinson’s disease (PD). However, the role of aging in the pathogenesis of PD is not known and it is currently uncertain why the symptoms take many decades to develop when inherited mutations that cause the disease can be present from birth. We hypothesize that there are specific changes that take place during the aging process that make cells susceptible to disease-causing mutations that are well-tolerated at younger ages. If so, then interventions that increase lifespan should be beneficial in the treatment of PD. To test this hypothesis, we used the powerful genetics of C. elegans, as this worm has been used extensively in aging research. We crossed transgenic worm models of PD expressing either human mutant α-synuclein (A53T) or LRRK2 (G2019S) with the long-lived insulin-IGF1 receptor mutant, daf-2. The daf-2 mutation increased the lifespan of both PD mutants. The increase in lifespan resulting from the daf-2 mutation rescued the degeneration of dopamine neurons in both worm models of PD and importantly rescued deficits in dopamine-dependent behaviors including basal slowing, ethanol avoidance, and area-restricted searching. Increasing lifespan through daf-2 mutation also delayed the formation of small aggregates in a worm model of PD expressing α-synuclein in the body wall muscle and rescued deficits in resistance to different stresses that were present in the PD mutant worms. Overall, this work suggests that slowing down the aging process may provide an effective treatment for PD.
Parkinson’s disease (PD) is the second most common neurodegenerative disease affecting as many as 10 million individuals worldwide. PD is characterized by deficits of movement, including resting tremor, bradykinesia, rigidity, postural instability, and shuffling gait. Patients with PD also exhibit non-motor symptoms that can include dementia, loss of smell, sleep disturbances, constipation, and depression. In the brain, PD is characterized by the degeneration of dopaminergic neurons within the substantia nigra (SN). The SN supplies dopamine to the striatum, thereby having an important role in movement. Brains of patients with PD also exhibit protein aggregates known as Lewy bodies. Although symptomatic treatments are available that can reduce motor deficits, there are currently no neuroprotective therapies available that can delay the progression of the disease.
While the pathogenesis of PD is incompletely understood, a number of genes and environmental factors have been implicated. The first gene to be linked to PD was SNCA, which encodes α-synuclein (α-syn).1 Interestingly, both mutations in the SNCA gene and increased copy number of wild-type α-syn lead to PD.2 Moreover, α-syn aggregates to form Lewy bodies.3 The most commonly mutated gene among PD patients is LRRK2, which encodes a Leucine Rich Repeat Kinase.4,5 Mutations in SNCA and LRRK2 give rise to an autosomal dominant form of PD and are thought to result from a toxic gain of function.
Aging is the greatest risk factor for the development of PD.6 Although the prevalence of PD is 0.3% in the general population, this number increases to 1% of those over 60 and 4% of individuals >80 years of age. Thus, in the inherited forms of PD, patients are symptom free for many decades despite the fact that the disease-causing mutation is present from birth. It is currently uncertain why the disease takes many decades to develop and the role of aging in the disease is poorly understood. We hypothesize that there are changes that take place during normal aging that make neurons susceptible to disease-causing mutations that were well tolerated at younger ages. This hypothesis is supported by the fact that disease onset in animal models of PD is proportional to the lifespan of the organism, indicating that the disease progresses according to biological age and not chronological time. In fact there are a number of changes that take place during normal aging that have been implicated in the pathogenesis of PD. These changes include protein aggregation,7 increased oxidative stress,8 decreased mitochondrial function,9 dysfunction of the proteasome,10 and impairment of autophagy.11
To test the role of aging in PD, we chose to use Caenorhabditis elegans models as these worms offer several advantages for the study of both aging and neurodegenerative disease. The first genes to increase lifespan in any organism were identified in C. elegans,12,
A number of worm models of PD have been generated through either exposing worms to a neurotoxic chemical such as MPP+ or 6-OHDA or by reproducing the genetic defect present in inherited forms of PD.18,
In this study, we chose to examine the effect of delaying aging in two worm models of PD to ensure that any beneficial outcomes we observe are not model specific. We use a genetic approach to delay aging in α-syn and LRRK2 worm models of PD by decreasing insulin-IGF1 signaling with a mutation in the insulin-IGF1 receptor gene daf-2. We find that delaying aging rescues multiple deficits present in both worm models of PD including the degeneration of dopamine neurons.
Worm models of Parkinson’s disease exhibit phenotypic abnormalities that can be used as outcome measures to assess the effect of delaying aging
Before examining the role of aging in PD, we first sought to determine what phenotypic abnormalities are present in worm models of PD that could be used as outcome measures. We choose to focus on α-syn and LRRK2 as both have been implicated in genetic and sporadic forms of PD. These worm models of PD express either human mutant α-syn with the A53T mutation (Pdat-1:: α-syn(A53T), which will be referred to as α-syn(A53T))20 or human mutant LRRK2 with the G2019S mutation (Pdat-1::LRRK2(G2019S),Pdat-1::GFP, which will be referred to as LRRK2(G2019S))21 exclusively in dopamine neurons under the dat-1 promoter. The LRRK2 worms were generated with the co-injection of a transgene expressing GFP in dopamine neurons (Pdat-1::GFP). Accordingly, we have used a strain expressing GFP in dopamine neurons as the control for the LRRK2 mutant, while we have used WT (N2) worms as the control for the α-syn mutants.
Examining the physiologic rates of the PD mutant worms we found that the α-syn mutants have normal lifespan, normal post-embryonic development time, normal fertility, normal movement (thrashing rate), a slower rate of defecation, and a decreased pharyngeal pumping rate (Figure 1a–f). α-syn mutants also exhibited significantly increased sensitivity to heat stress, normal sensitivity to osmotic stress, and increased sensitivity to oxidative stress (Figure 1g–i). Finally, we examined the ability of α-syn worms to perform three dopamine-dependent behaviors: basal slowing,25 ethanol avoidance,26 and area-restricted searching.27 Worms with a mutation in the tyrosine hydroxylase gene cat-2, which have depleted levels of dopamine,28 exhibit marked deficits in all three behaviors. α-syn mutant worms exhibited deficits in all three dopamine-dependent behaviors (Figure 1j–l), suggesting that the expression of mutant α-syn in dopamine neurons disrupts dopamine signaling in these worms.
Compared with Pdat-1::GFP control worms, LRRK2 mutant worms exhibit a normal lifespan, normal development time, markedly decreased fertility, a trend towards increased thrashing rate, a more rapid rate of defecation, a normal rate of pharyngeal pumping, increased sensitivity to heat stress, normal sensitivity to osmotic stress, and normal sensitivity to oxidative stress (Figure 1a–i). As with α-syn mutant worms, LRRK2 mutants show deficits in dopamine-dependent behaviors including an inability to basal slow and lack of ethanol avoidance (Figure 1 j–l). Examination of worms expressing WT α-syn or WT LRRK2 revealed that these worms also exhibit some of the phenotypic deficits observed in the mutant strains (Supplementary Figure S1), although the magnitude of the deficit tended to be milder than worms expressing the mutant form of these proteins (Supplementary Table S1).
As the PD mutant worms exhibited differences from WT in pharyngeal pumping, resistance to heat stress and defecation cycle rate, we sought to determine the extent to which these phenotypes might be dopamine dependent. For this purpose we tested cat-2 tyrosine hydroxylase mutants and found that cat-2 worms exhibit normal defecation and heat stress resistance but decreased pharyngeal pumping (Supplementary Figure S2). This suggests the possibility that the toxicity of mutant α-syn and LRRK2 may cause deficits that are independent of dopamine signaling.
Overall, both α-syn and LRRK2 mutant worms exhibit multiple phenotypic abnormalities, which can be used as outcome measures to identify disease modifiers.
Decreasing insulin/IGF1 signaling increases lifespan in worm models of Parkinson’s disease
Having identified phenotypic differences that can be used as outcome measures to assess the role of aging in PD, we used a genetic approach to determine the effect of delaying aging in the two worm models of PD. We crossed the α-syn and LRRK2 transgenic worms to long-lived daf-2 worms. daf-2 worms live twice as long as wild-type worms as a result of decreased insulin-IGF1 signaling.12
Before examining the effect of the daf-2 mutation on the abnormal phenotypes present in these worm models of PD, we first wanted to ensure that the daf-2 mutation was able to increase lifespan in the two PD mutants. We found that α-syn(A53T) worms live as long as wild-type worms and that the double mutant α-syn(A53T);daf-2 worms exhibited increased lifespan compared with α-syn(A53T) worms, thereby indicating that the daf-2 mutation had the intended effect of delaying aging in α-syn(A53T) worms (Figure 2a). Similarly, we found that LRRK2(G2019S) worms have a normal lifespan and that their lifespan is increased by the daf-2 mutation (Figure 2b). As an additional measure of slowing aging we monitored the accumulation of lipofuscin with age. Lipofuscin is a product of oxidative damage that accumulates with age and has been used as a marker of aging. We found that in both α-syn(A53T);daf-2 worms and LRRK2;daf-2 worms there was a markedly slower accumulation of lipofuscin than in α-syn(A53T) and LRRK2 mutants (Supplementary Figure S3). This indicates that the daf-2 mutation is effective in delaying aging in both PD mutants.
Delaying aging increases the survival of dopamine neurons in worm models of Parkinson’s disease
Having shown that the daf-2 mutation could delay aging in both PD mutants, we next sought to determine whether delaying aging would have a beneficial effect on the abnormal phenotypes present in these strains. As PD is characterized by the selective loss of dopamine neurons in the SN, we first examined the degeneration of dopamine neurons with increasing age. As has been previously reported,21,29 we found that there is a slow degeneration of dopamine neurons with increasing age in wild-type worms that is accelerated by expression of α-syn(A53T) or LRRK2(G2019S; Supplementary Figure S5). Comparing α-syn(A53T) worms and α-syn(A53T);daf-2 worms, we found that the daf-2 mutation resulted in a significantly slower rate of dopamine neuron loss with age (Figure 2c). Similarly, the degeneration of dopamine neurons was markedly less in LRRK2(G2019S);daf-2 worms than in LRRK2(G2019S) worms (Figure 2d,e). In fact, at day 30, when all of the LRRK2(G2019S) worms have died, LRRK2(G2019S);daf-2 worms have a similar number of dopamine neurons to LRRK2(G2019S) worms on day 5. Combined this indicates that delaying aging can markedly slow the degeneration of dopamine neurons in worm models of PD.
We also examined the dendrites of dopamine neurons for signs of degeneration prior to the loss of the neuronal cell body. We quantified dendritic blebs (see Supplementary Figure S6 for image) and found that these blebs increased with age and were found more frequently in LRRK2(G2019S) PD mutants (Supplementary Figure S6).
Delaying aging improves dopamine dependent behaviors in worm models of Parkinson’s disease
Having shown that delaying aging through the daf-2 mutation is neuroprotective in worm models of PD, we next sought to determine the extent to which neuronal function is preserved. To do this, we examined the ability of the daf-2 mutation to rescue deficits in dopamine-dependent behaviors. We found that while both α-syn(A53T) or LRRK2(G2019S) mutants exhibit little or no basal slowing, α-syn(A53T);daf-2 and LRRK2(G2019S);daf-2 demonstrate basal slowing that is indistinguishable from wild-type (Figure 3a and b). Similarly, despite the fact that neither PD mutant strain showed any degree of ethanol avoidance, in both cases the daf-2 mutation partially restored function towards wild-type (Figure 3c and d). Finally, in the area-restricted searching assay, we found that both α-syn(A53T);daf-2 and LRRK2(G2019S);daf-2 mutants exhibited increased searching compared with α-syn(A53T) and LRRK2(G2019S) single mutants, respectively (Figure 3e and f). Thus, in addition to preserving the number of GFP-positive dopamine neurons in PD mutant worms, delaying aging through the daf-2 mutation also has a functional impact in preventing the loss of dopamine-dependent behaviors.
We also examined the effect of the daf-2 mutation on physiologic rates in the α-syn and LRRK2 PD mutant worms. We found that delaying aging through mutation of daf-2 did not improve fertility (Supplementary Figure S7a,b), pharyngeal pumping rate (Supplementary Figure S7c,d), or thrashing rate (Supplementary Figure S7e,f) in either PD mutant. Interestingly, the expression of LRRK2(G2019S) in dopamine neurons significantly increased the rate of movement of daf-2 mutant worms (Supplementary Figure S7f).
Delaying aging rescues deficits in resistance to stress in worm models of Parkinson’s disease
Increasing lifespan through mutations in daf-2 has been shown to increase resistance to a variety of stresses including heat stress,30 oxidative stress,31 and osmotic stress.32 As both PD mutants exhibited increased sensitivity to different types of stress, we next determined the extent to which increasing lifespan through the daf-2 mutation could rescue the deficits in stress resistance in α-syn and LRRK2 transgenic worms. Both α-syn and LRRK2 mutants exhibit increased sensitivity to heat stress (Figure 4a and b). In both cases the deficit was completely rescued in the daf-2 double mutant (Figure 4a and b). Similarly, the increased sensitivity to oxidative stress that is present in α-syn(A53T) mutant worms is ameliorated by the daf-2 mutation (Figure 4c). Finally, we found that delaying aging through daf-2 mutation also improved resistance to oxidative stress in LRRK2(G2019S) mutant worms and osmotic stress resistance in both α-syn and LRRK2 PD worm models (Figure 4d and f).
Delaying aging decreases the formation of small α-synuclein aggregates
As PD is characterized by the formation of α-syn aggregates called Lewy bodies, we next sought to determine whether delaying aging would also decrease aggregation. To be able to visualize aggregation in live worms, we utilized a worm model of PD in which wild-type α-syn is linked to yellow fluorescent protein (YFP) for easy visualization and expressed in body wall muscle under the unc-54 promoter (Punc-54:: α-syn(WT):YFP), which will be referred to as BW-α-syn worms. These worms have previously been shown to exhibit aggregation that increases with age.24 We crossed the BW-α-syn worms with daf-2 mutants in order to delay aging (Figure 5a) and examined the formation of aggregates with increasing age. Unlike worms expressing a mutant length of polyglutamine linked to YFP under the same unc-54 promoter, which exhibit large aggregates, BW-α-syn have smaller aggregates of varying sizes (Supplementary Figure S8). To compensate for this heterogeneity, we used two different paradigms: (1) we quantified aggregates that could be seen under low magnification (dissecting fluorescent microscope) in whole worm images and (2) we quantified aggregates in a defined area surrounding the vulva under high magnification (compound fluorescent microscope). We found that while the daf-2 mutation had little impact on the number of aggregates that could be visualized in whole worms (Figure 5b), it resulted in a significant decrease in smaller aggregates surrounding the vulva (Figure 5c).
As BW-α-syn PD mutant worms exhibit deficits in osmotic stress resistance and movement, we next examined whether daf-2 mutation would be able to rescue these deficits. We found that the markedly decreased survival of BW-α-syn worms under osmotic stress (500 mM NaCl) was completely rescued in BW-α-syn;daf-2 double mutants such that the double mutants survived better than wild-type (Figure 5d). Similarly, we found that BW-α-syn worms have decreased movement in a thrashing assay (Figure 5e and f). Despite the fact that daf-2 mutation results in decreased movement on a wild-type background, the daf-2 mutation significantly improved movement in BW-α-syn mutant worms (Figure 5e and f). In fact, the rate of movement in BW-α-syn;daf-2 worms and daf-2 worms was indistinguishable.
Decreasing levels of FOXO transcription factor DAF-16 prevents the beneficial effects of daf-2 mutation in LRRK2 worm model of Parkinson’s disease
The insulin-IGF1 receptor encoded by the daf-2 gene modulates gene expression by controlling the nuclear localization of the FOXO transcription factor DAF-16. Accordingly, the ability of the daf-2 mutation to increase lifespan is entirely dependent on DAF-16.12 To determine whether signaling through DAF-16 is required for the beneficial effect we observe in worm models of PD, we used RNAi to knockdown DAF-16 levels in LRRK2(G2019S);daf-2 worms. We found that daf-16 RNAi was effective at knocking down DAF-16:GFP expression in a Pdaf-16:daf-16:GFP reporter strain (Supplementary Figure S9a). However, we noticed that there was still some residual DAF-16:GFP expression in neurons, which is consistent with previous observations that RNAi is less efficient in neurons.
To assess the impact of daf-16 RNAi on the ability of the daf-2 mutation to increase longevity in LRRK2(G2019S) worms, we examined lifespan and lipofuscin accumulation. We found that daf-16 RNAi completely abolished the increased lifespan resulting from daf-2 mutation (Figure 6a). Similarly, lipofuscin accumulation was greater in daf-16 RNAi treated worms suggesting that the ability of the daf-2 mutation to delay aging was inhibited by our daf-16 RNAi treatment paradigm (Supplementary Figure S9b).
Having shown that daf-16 RNAi could prevent the beneficial effect of daf-2 mutation on lifespan, we next sought to determine if daf-16 RNAi would also prevent the amelioration of phenotypic abnormalities observed in LRRK2(G2019S);daf-2 PD mutants. We found that daf-16 RNAi reduced the beneficial effect of daf-2 mutation on ethanol avoidance, area-restricted searching, osmotic stress resistance, heat stress resistance, dendritic blebs, and loss of dopamine neurons (Figure 6). In contrast, daf-16 RNAi did not worsen basal slowing or oxidative stress resistance in LRRK2(G2019S);daf-2 worms (Figure 6b and g). To determine whether this might be due to the residual DAF-16 expression that we observed in neurons, we generated LRRK2(G2019S);daf-2;daf-16 triple mutant worms. We found that the daf-16 mutation prevented the improvement in basal slowing and completely abolished the improved resistance to oxidative stress in LRRK2(G2019S);daf-2 worms (Figure 6b and g). Overall, this indicates that the beneficial effect of daf-2 mutation in worm models of PD is mediated by DAF-16.
Aging and Parkinson’s disease
Aging is the greatest risk factor for PD.33 Advancing age not only increases the likelihood that an individual will develop PD,6 but those that develop PD at a later age have a more severe disease course in terms of motor impairment, levodopa responsiveness, gait and postural deficits, and dementia.34 In fact, there are many commonalities between PD and the normal process of aging (for a comprehensive summary see Table 1 in ref. 35). The pattern of selective cell loss in the brain is similar between PD and aging.33 Accumulation of α-syn protein occurs with advancing age and in PD.36 Both aging and PD are believed to be caused by a complex combination of genes and environmental factors, with relatively few genes having major effects.37 In addition, many of the changes that take place during normal aging, have been implicated in the pathogenesis of PD including increased aggregation,7 increased oxidative stress,8 decreased mitochondrial function,9 dysfunction of the proteasome,10 and impairment of autophagy.11 On the basis of the large number of similarities between aging and PD, it has been proposed that PD may result from aging.35 If so, then delaying aging may be an effective strategy to treat PD. Our results provide a proof of principle that delaying aging can be neuroprotective in PD.
Worm models of Parkinson’s exhibit loss of dopamine neurons and deficits in dopamine-dependent behaviors
In the characterization of α-syn and LRRK2 mutant worms, we were able to reproduce originally reported phenotypes in these strains20,21 and to identify novel deficits. All of the phenotypes present in these strains result from the expression of the mutant protein in the eight dopamine neurons present in the worm (it is possible that the dat-1 promoter drives low level of expression in other tissues). This comprises a small fraction of the 302 neurons and 959 cells that are present in the worm. The loss of dopamine neurons in the SN is a characteristic feature of PD. It has also been shown that the number of dopamine neurons declines with age in unaffected individuals albeit at a decreased rate compared with PD. Similarly, we found that GFP-positive dopamine neurons were lost with increasing age in wild-type worms and the rate of loss is accelerated in both PD mutants. We also observed deficits in multiple dopamine-dependent behaviors including basal slowing, ethanol avoidance, and area-restricted searching. We have observed similar deficits in cat-2 mutant worms that have a mutation in the gene encoding tyrosine hydroxylase. As tyrosine hydroxylase is required for the synthesis of dopamine, the cat-2 worms have decreased levels of dopamine. Similarly, dopamine levels have previously been shown to be decreased in both the α-syn and LRRK2 worms models used in our study.20,21
Our results show an increased sensitivity to heat stress in both α-syn and LRRK2 mutants, as well as an increased sensitivity to oxidative stress in α-syn mutant worms. This is surprising given that the expression is limited to the eight dopamine neurons. Nonetheless, this is consistent with studies on aging showing that specific neurons can modulate survival in response to temperature.38 We also observe a marked decreased in fertility in LRRK2 mutants. Previous studies have shown that exogenous dopamine inhibits egg laying.39 As LRRK2(G2019S) mutants have decreased levels of dopamine,21 perhaps endogenous, and exogenous dopamine have different effects on egg laying.
The fact that α-syn and LRRK2 mutants exhibit deficits in defecation cycle length and heat stress resistance that are not observed in cat-2 mutants, which have diminished levels of dopamine, suggests the possibility that these may be dopamine-independent deficits resulting from α-syn and LRRK2 toxicity. There are multiple possibilities that could explain the additional deficits present in the PD worms. First, the expression of a toxic protein such as LRRK2 or α-synuclein could disrupt a function of the CEP, ADE, or PDE neurons that is not mediated by dopamine. Second, the expression of a toxic protein such as LRRK2 or α-synuclein could cause the dopamine neurons to release chemokines that negatively influence neighboring cells. Third, at least in the case of the α-synuclein mutants, there may be prion-like transfer to other non-dopamine neurons that may contribute to these phenotypes.
Delaying aging by mutation of daf-2 is beneficial in worm models of Parkinson’s disease
In this study, we focused on the insulin-IGF1 signaling pathway as a means of delaying aging in worm models of PD. The daf-2 gene encodes the insulin-IGF1 receptor and mutations in this gene have been shown to more than double lifespan in the worm.12 After the insulin-IGF1 signaling pathway was shown to increase lifespan in C. elegans, genes in this same pathway were found to increase lifespan in yeast, flies and mice, thereby indicating conservation across species.40 Importantly, genes in this same pathway have been shown to be associated with longevity in humans.17
We found that delaying aging through the mutation of daf-2 is neuroprotective in two different genetic models of PD. In fact, LRRK2(G2019S);daf-2 double mutants have more dopamine neurons remaining at day 30 (10 days past the average lifespan of LRRK2(G2019S) and WT worms) than LRRK2(G2019S) mutants have on day 8 of adulthood. Although the rate of neuronal loss in α-syn(A53T) transgenic worms is decreased compared with LRRK2(G2019S) worms, there is still a significant rescue imparted by the daf-2 mutation. We also found that delaying aging rescued deficits in dopamine-dependent behaviors and abolished the increased sensitivity to stress observed in the PD mutants. We did not observe any beneficial effect on the reduced fertility present in LRRK2(G2019S) mutants, but perhaps this is due to the fact that the daf-2 mutation decreases brood size in wild-type worms. While we were completing our study, the Caldwell group showed a beneficial effect of the daf-2 mutation in a different α-syn model of PD.41 In their study, they utilized a transgenic worm expressing wild-type α-syn and found that a mutation in daf-2 could rescue dopaminergic degeneration and decrease aggregation in body wall muscle. The fact that two independent experiments in different labs with different models both show a beneficial effect of delaying aging in worm models of PD provides strong support that this may be an effective target for treating PD. In addition, a screen for modifiers of α-syn aggregation identified multiple aging genes that were able to suppress aggregate formation.24
Further support for this strategy comes from experiments showing a beneficial effect of interventions that increase lifespan in chemically induced rodent models of PD. Resveratrol, a potent enhancer of the histone deacetylase Sirtuin 1 activity that has been shown to increase lifespan in worms, flies, and mice,42 has been shown to be protective in the 6-OHDA rat model of PD.43 Rapamycin, an inhibitor of mTOR signaling that increases lifespan in mice,44 was shown to be protective in the MPTP mouse model of PD.45 Dietary restriction, which has been shown to increase lifespan in yeast, worms, flies, mice, and monkeys,46 improved survival of dopamine neurons in MPTP-treated rodents47 and resulted in better maintenance of motor activity in MPTP-treated primates.48 Finally, treatment with the anti-diabetic drug metformin has been shown to increase lifespan in worms and mice49,50 and has been found to improve neuronal survival, motor function, and behavior following MPTP treatment in mice.51 Overall, the fact that multiple interventions that increase lifespan exhibit a beneficial effect in PD suggests that targeting the aging process may be an effective strategy for treating PD.
Targeting aging in mouse models of PD and PD patients
Whereas there is a single insulin-IGF1 receptor in C. elegans, in mice and humans there are separate receptors for insulin and IGF1. Nonetheless, evidence from a number of mouse models indicates that decreasing either insulin or IGF1 signaling can lead to increased lifespan in mice as well. Mice bearing a heterozygous deletion in the IGF1 receptor gene Igf1r are long lived,16 as are mice with a homozygous deletion in the insulin receptor that is limited to adipose tissue.52 Mice with a heterozygous deletion in the insulin receptor substrate 2 gene (Irs2), either throughout the body or limited to just the brain, are also long lived.53 Long-lived Snell dwarf mice, Ames dwarf mice, and growth hormone receptor mutants have all been shown to have decreased levels of IGF1.54,
In translating the results from the present study to mice and eventually humans, it will be essential to determine in which tissue(s) insulin-IGF1 signaling must be decreased in order to have a beneficial effect in PD. Decreasing insulin or IGF1 signaling in mammals may be complicated by potential detrimental side effects. For example, loss of insulin signaling in the pancreas could lead to diabetes. However, if the neuroprotective effect of the daf-2 mutation is cell autonomous, then it may be possible to reduce insulin signaling specifically in dopamine neurons, thereby avoiding or minimizing the possibility of side effects. As it has previously been shown that decreasing insulin-IGF1 signaling in neurons is required for the long lifespan of daf-2 mutants,58 it is possible that reducing insulin-IGF1 signaling in neurons will be sufficient to protect the neurons from the toxic effects of mutant α-syn or LRRK2.
One previous study examined the effect of decreasing IGF1 signaling in a mouse model of PD. Heterozygous Igf1r+/− mice were treated with MPTP and were found to have a larger lesion than WT controls.59 Although this result appears to contradict the results from our study in C. elegans, it should be noted that the Igf1r+/− mice only have a mild increase in lifespan and the MPTP model involves an acute exposure to highly toxic chemical. This model recapitulates the neuronal loss present in PD, but does not reproduce the pathogenesis of the disease. Thus, it is possible that delaying aging through decreasing insulin or IGF1 signaling may be beneficial in a genetic mouse model of PD that more accurately reproduces the pathogenic mechanisms underlying PD. Support for this conclusion comes from the fact that decreasing insulin or IGF1 signaling has previously been shown to be beneficial in genetic mouse models of other neurodegenerative diseases including Alzheimer’s disease60 and Huntington’s disease.61
Overall, we show that delaying aging through decreasing insulin-IGF1 signaling is neuroprotective in worm models of PD. Future studies will need to validate these results in genetic mouse models of PD. As decreasing insulin or IGF1 signaling may have detrimental effects in humans it may be necessary to target specific tissues and tightly control the degree to which signaling is knocked down. As an alternative approach, it may be fruitful to explore other pathways of lifespan extension, which are less likely to induce side effects.
Materials and methods
C. elegans strains and maintenance
The following strains were used in this study:
CB1370 daf-2(e1370) III,
JVR120 daf-16(mu86) I,
JVR103 Pdat-1:: α-synuclein[WT],
JVR203 Pdat-1::α-synuclein[A53T]; vtIs7[pDAT::GFP(pRB490)],
JVR206 daf-2(e1370) III; vtIs7[pDAT::GFP(pRB490)],
JVR205 daf-2(e1370) III; Pdat-1:: α-synuclein[A53T],
JVR210 daf-2(e1370) III; Pdat-1:: α-synuclein[A53T]; vtIs7[pDAT::GFP(pRB490)],
JVR105 cwrIs730 [Pdat-1::GFP, lin-15(+)],
JVR189 daf-2(e1370) III; cwrIs730 [Pdat-1::GFP, lin-15(+)],
JVR104 cwrIs856 [Pdat-1::GFP, Pdat-1::LRRK2(WT), lin-15(+)],
JVR168 cwrIs722 [Pdat-1::GFP, Pdat-1::LRRK2(WT), lin-15(+)],
JVR202 daf-2(e1370) III; cwrIs722 [Pdat-1::GFP, Pdat-1::LRRK2(WT), lin-15(+)],
NL5901 pkIs2386[punc-54:: α-synuclein::YFP+unc-119(+)],
JVR192 daf-2(e1370) III; pkIs2386[punc-54:: α-synuclein::YFP+unc-119(+)],
JVR323 daf-16(mu86) I; daf-2(e1370) III; cwrIs722 [Pdat-1::GFP, Pdat-1::LRRK2(WT), lin-15(+)].
All strains were maintained at 16 °C to prevent dauer formation in the daf-2 mutant strains. Worms were shifted to 20 °C on day 1 of adulthood for the completion of phenotyping assays. Strains were outcrossed to our N2 strain six times to obtain a uniform strain background.
Generation of double mutants
Double mutants were generated by standard techniques. In most cases, N2 males were crossed to GFP/YFP positive worms (e.g., Pdat-1::GFP). Fluorescent males from the progeny were crossed to a deletion mutant (e.g., daf-2). The resulting fluorescent hermaphrodites (e.g., daf-2/+; Pdat-1::GFP/+) were selfed. Eight fluorescent progeny was then singled and the genotype determined by PCR for deletion mutants or sequencing for point mutants. In the case of daf-2 crosses, eggs and L1 worms from the second cross were transferred to 25 °C. After 2–3 days, dauers were transferred to a new plate. After an additional day at 25 °C, worms that were still dauer were recovered at 16 °C, singled onto individual plates and the genotype of the worm was confirmed by sequencing. Homozygosity of fluorescent transgenes was determined by counting 30 worms in three consecutive generations and observing 100% fluorescence.
Blinding of experimenters and replicates
All studies were completed such that the experimenter was blind to the genotype of the worms. Strains were given letter codes by another member of the laboratory and the code was not broken until all of the replicates for a particular assay were completed. For all assays, we completed a minimum of three biological replicates per strain.
For RNAi experiments, individual colonies from freshly streaked LB-Tetracycline-Ampicillin plates were grown for 10–12 h in LB media containing 50 μg/ml carbenicillin. Bacteria was concentrated fivefold and seeded onto NGM plates containing 1 μg/ml IPTG and 50 μg/ml carbenicillin. After 2 days of induction, L4 worms were transferred to RNAi plates. The next day gravid adults were transferred to a new plate. These adults were removed the next day and their progeny were used for experiments.
Lifespan was measured on plates containing 25 μM 5-fluoro-2′-deoxyuridine (FUdR) to limit the growth of progeny. This concentration was shown to have minimal effects on lifespan.62 As this concentration of FUdR does not completely prevent the development of progeny to adulthood in the first generation, worms were transferred to fresh plates after 4 days. Thereafter, worms were transferred to fresh plates weekly. Viability was assessed every 2 days by gentle prodding with a platinum pick. Worms that either had internal hatching of progeny or expulsion of internal organs were not counted as deaths.
Postembryonic development time
Post-embryonic development (PED) time was measured by transferring eggs to an NGM plate. After 3 h, newly hatched L1 worms (20 worms per replicate) were transferred to a new NGM plate. The time from hatching to the L4-adult transition was measured as the PED time.
Brood size was measured by placing individual worms at the L4 stage onto NGM plates followed by daily transfers to new plates. The resulting progeny was allowed to develop to adulthood before counting (5 worms per replicate).
Rate of movement
Rate of movement was assessed by measuring thrashing in liquid using video-tracking and computer analysis. Approximately 50 worms were placed in M9 buffer (22 mM KH2PO4, 34 mM K2HPO4, 86 mM NaCl, 1 mM MgSO4) on a clean NGM plate. Videos were taken with an Allied Vision Tech Stingray F-145 B Firewire Camera (Allied Vision, Exton, PA, USA) at 1024×768 resolution, 8-bit using the MATLAB image acquisition toolbox. Analysis was performed using wrMTrck plugin for ImageJ (publically available at http://www.phage.dk/plugins).
Defecation cycle length was determined by measuring the time between two consecutive pBoc contractions in day-1 adult worms with at least 5 worms per replicate. To minimize the effects of laboratory temperature, defecation was measured on water filled chambers that had been incubated at 20 °C and the lids of the plates containing the worms were not removed.
Pharyngeal pumping rate
Pharyngeal pumping rate was assessed by video-recording followed by manual counting in day-1 adult worms with 10 worms per replicate. For each measurement worms were placed on an OP50 bacteria-seeded NGM assay plate and recorded for 30 s. Recordings taken at 15 frames per second were replayed at half speed for manual counting.
Stress resistance assays: Heat stress, Oxidative stress, Osmotic stress
Sensitivity to heat stress was determined by assessing survival of young adult worms incubated at 35 °C. Survival was assessed hourly. Sensitivity to oxidative stress was determined through multiple paradigms. Sensitivity to acute oxidative stress was assessed through exposure to increasing concentrations of juglone (Sigma, St. Louis, MO, USA). Young adult worms were transferred to freshly prepared NGM plates containing 240 μM juglone, and survival was assessed hourly. Sensitivity to chronic oxidative stress was determined through exposure to plates containing 2 mM paraquat (methyl viologen, Sigma) beginning at day-1 of adulthood. FUdR (100 μM) was added to these plates to prevent internal hatching of progeny. Survival was monitored daily until death. Sensitivity to osmotic stress was determined by transferring young adult worms to NGM plates containing increased concentrations of NaCl (450–500 mM). The survival of worms was determined after 48 h. All stress assays were completed on day-1 of adulthood and included a minimum of 20 worms per replicate.
Approximately 50 worms at day 3 of adulthood were washed in M9 buffer to remove any residual bacteria. The cleaned worms were then transferred to either unseeded NGM plates or NGM plates seeded with OP50 bacteria covering the entire plate. After 5 min, videos of the entire plate were recorded for 1 min with an Allied Vision Tech Stingray F-504 B Firewire Camera and a Navitar Zoom 7000 lens (Navitar, Tokyo, Japan) using and the MATLAB image acquisition tool. Recordings were processed using the wrMTrck plugin for ImageJ. Basal slowing was calculated as the difference in rate of movement on food versus off food divided by the rate of movement off food.
Ethanol avoidance assay
Day-1 adult worms were transferred to assay plates, which are divided into four quadrants: two quadrants seeded with 50 μl ethanol and the others without. Worms are placed in the center of the assay plate and allowed to move for 30 min at which point the entire plate is imaged and the worms are scored for their quadrant of preference. Ethanol avoidance is calculated as ((number of worms in control quadrants)−(number of worms in ethanol quadrants))/ total number of worms.
Twenty well-fed day-1 adult worms were placed on a clean 60 mm NGM assay plate. One-minute-long video-recordings were taken at 5 min and 30 min after transfer to the assay plate. The tracks of individual worms are then analyzed for the number of turns exceeding 90° are counted. The area-restricted searching ratio is calculated as the number of turns per worm at 5 min divided by the number of turns per worm at 30 min. A minimum of three replicates per strain were completed.
Synchronized worms at either day 6 or day 9 of adulthood were plated on NGM plates and aged to the appropriate time point. Worms were then transferred to a clean 60mm NGM plate and paralyzed using 2 mM levamisole. Whole-worm images were captured using a Nikon SMZ 1500 dissecting microscope (Tokyo, Japan) with an Allied Vision Tech Stingray F-145 B Firewire Camera using Vimba image acquisition software (Allied Vision, Exton, PA, USA).
Degeneration of dopamine neurons and quantification of dendritic blebs
The degeneration of dopamine neurons was monitored by expressing GFP specifically in dopamine neurons under the dat-1 dopamine transporter promoter. It was previously shown that treatments that cause a loss of GFP-positive neurons cause a corresponding loss of dopamine neuron cell bodies.63 Synchronized Pdat-1:GFP worms were plated onto 25 μM FUdR agar plates to be observed at increasing ages. At each time point 10–15 worms were mounted onto a 1% agar pad on a glass slide, immobilized using 2 mM levamisole, and enclosed with a coverslip. Imaging of immobilized animals was carried out with an Axioplan 2 inverted fluorescence microscope (Zeiss, Oberkochen, Germany). Quantification of dopamine neurons and dendritic blebs was done in a blinded manner.
Measurement of aggregation
Localized aggregate counts
Worms were mounted onto slides as described above. Fluorescent punctae were then manually counted in a defined region centered around the vulva using a ×63 objective on a Zeiss Axioplan 2 compound microscope (Zeiss, Oberkochen, Germany).
Whole-worm aggregate measurements
Whole-worm images were captured as described for lipofuscin measurements. Punctae, defined as clusters of at least 3 pixels whose intensity were at least 1 standard deviation above the background intensity, were quantified using MATLAB.
We thank Shu Chen for providing us with the LRRK-2 transgenic strain and Takeshi Iwatsubo and Shohei Mitani for providing us with the α-synuclein transgenic strain. We also thank Richard Nass and David Blakely for providing us with the BY250 strain and Tim Feinstein for helping us with confocal imaging of dopamine neurons. Some strains were provided by the CGC, which is funded by NIH Office of Research Infrastructure Programs (P40OD010440). This work was supported by the Van Andel Research Institute and Parkinson Society of Canada. JC and EM are supported by the Van Andel Institute Graduate School.