Longevity WG short report

Longevity Working Group Evaluation Team: Jason Colasanti, Aaron King, Estéfano Pinilla, Anonymous member

Project PI: Prof. Viktor Korolchuk (Staff Profile - Faculty of Medical Sciences - Newcastle University)

Project Page on Molecule

Simple Summary

Ageing is associated with the decline in the capacity of the autophagy pathway to degrade dysfunctional and damaging cellular components, such as protein aggregates and mitochondria. Dysfunctional autophagy, in turn, undermines other cellular functions including DNA repair, metabolism and survival. Therefore, activation of autophagy is considered a promising therapeutic approach to combat ageing and age-related diseases. A large number of screens has been performed and published to date, these have identified a wide range of small molecules that stimulate initiation of autophagy. Prof. Korolchuck lab proposes to initiate a drug discovery programme with the aim of identifying novel bioactive autophagy inducers.

Problem

Lysosomal dysfunction is an important factor contributing to the reduction of autophagy during aging. As dysfunctional lysosomes interfere with autophagy at the terminal stage, stimulation of autophagy initiation can be ineffective to rescue autophagy. Additionally, current methods to measure autophagy are rather unreliable, slow, and with complicated readouts, making the screening of compounds that promote autophagy less efficient.

Opportunity

To model lysosomal dysfunction, Prof. Korolchuk lab uses cells with a mutation in a lysosomal protein (Npc1) associated with neurodegenerative diseases. When these cells are subjected to metabolic stress, they suffer cell death due to dysfunctional autophagy, providing an easy readout for an autophagy assay (cells dead/cells alive). To identify true autophagy activators, Prof. Korolchuk lab uses cells that lack initiation of autophagy and are therefore not rescuable by autophagy inducers in parallel with Npc1 KO cells.

If funded by VitaDAO, Prof. Korolchuk lab will use this innovative method to screen an unique library of natural compounds, synthesize derivatives based on hits and identify their biological target.

Highlights

• Assay with easy readout, decent throughput, good controls and targeting one of the most important processes in cellular aging (autophagy)
• Solid evidence supporting their approach
• Small ticket size ($150000-$250000)
• The platform would allow collaboration with other projects targeting autophagy/mitophagy
• Potential for generation of IP/NFT for compounds coming out of their screening platform
• Strong and productive scientific team interested in the IP/NFT model and in company formation

Risks

• Current application relies on the screening of their current library of natural compounds producing hits, contingency plan needs to be planned with Prof. Korolchuk lab
• The screening model relies on rescuing autophagy in a single knockout model. A risk would be that they could be screening to solve a problem caused by this specific knockout that, although linked with some neurodegenerative diseases, lacked relevance in general aging. However, the team is working on addressing such risk and there are promising data suggesting this might not be a problem.

Outcome of the evaluation and recommendation

A total of 4 evaluators independently scored the project proposal on different categories as either: (1) Oustanding, (2) Strong, (3) Satisfactory, (4) Weak, (5) Unacceptable, (N/A) Not enough information provided, or (N/A) Not my area of expertise. This is a summary of the results:

• Novelty and Impact: (2) Strong (4/4 evaluators)
• Feasibility and Data: (1) Outstanding (3/4 evaluators); (3) Satisfactory (1/4 evaluators)
• Relevance to longevity: (1) Outstanding (1/4 evaluators); (2) Strong (2/4 evaluators); (3) Satisfactory (1/4 evaluators)
• Science Team: (2) Strong (3/4 evaluators); (3) Satisfactory (1/4 evaluators)
• Market Advantage: (2) Strong (1/4 evaluators); (3) Satisfactory (2/4 evaluators); (4) Weak (1/4 evaluators)
• IP-NFT Potential: (2) Strong (1/4 evaluators); (3) Satisfactory (2/4 evaluators); (N/A) Not enough information provided (1/4 evaluators)

All the evaluators consider the project worth funding by the VitaDAO community.

Mechanism of Funding

This proposal recommends VitaDAO commits funding via an IP-NFT.

Project proposal

Background

Ageing is associated with the decline in the capacity of the autophagy pathway to degrade dysfunctional and damaging cellular components, such as protein aggregates and mitochondria. Dysfunctional autophagy, in turn, undermines other cellular functions including DNA repair, metabolism and survival. Therefore, activation of autophagy is considered a promising therapeutic approach to combat ageing and age-related diseases. A large number of screens has been performed and published to date, these have identified a wide range of small molecules that stimulate initiation of autophagy.

However, lysosomal dysfunction is one of the prominent factors contributing to ageing and a driver of many age-related pathologies. In the presence of dysfunctional lysosomes, the autophagy pathway becomes blocked at the terminal stage. As such stimulation of autophagy initiation may not always be an effective approach to induce the flux through the system. We model this situation using cells with a mutation in a lysosomal protein Npc1 (mutations of which are associated with Niemann-Pick type C1 Disease and Parkinson’s Disease), which leads to the block in autophagosome degradation (Impaired autophagy in the lipid storage disorder Niemann–Pick type C1 disease - PMC).

Project Summary

Extensive work leading to this proposal identified a unique phenotype of cells with dysfunctional autophagy in tissue culture (Autophagy promotes cell survival by maintaining NAD(H) levels | Research Square, https://www.biorxiv.org/content/10.1101/2020.01.31.928424v1, under revision for Nat Cell Biol). In normal glucose-containing medium autophagy KOs upregulate glycolysis at the expense of mitochondrial respiration. When glucose is replaced with galactose, which results in zero net ATP production through glycolysis and cells are forced to respire, autophagy deficient cells become apoptotic. This phenotype is common for Npc1 KO MEFs where autophagosome maturation is impaired as well as for cells with the loss of core autophagy genes (Atg5, Atg7 and FIP200/Rb1cc1).

We established the sequence of events leading to cell death of autophagy deficient cells: 1) accumulation of dysfunctional mitochondria; 2) stress in the form of increased ROS and DNA damage; 3) activation of stress response pathways (NADases of Sirtuin and PARP family); 4) depletion of cellular NAD+ (and NADH) pools; 4) mitochondrial depolarisation; 5) apoptotic cascade. Our data with yeast, fly, and human stem cell-derived neuronal models of autophagy deficiency indicate that the mechanisms of cell death described in MEFs is evolutionarily conserved from yeast to humans (Autophagy promotes cell survival by maintaining NAD(H) levels | Research Square, https://www.biorxiv.org/content/10.1101/2020.01.31.928424v1).

Targeting the processes downstream of autophagy dysfunction (mitochondrial dysfunction, hyperactivity of NADases, NAD boosting, mitochondrial re-polarisation) can rescue cell death in cells/organisms with both the genetic loss of Atg genes and Npc1. On the other hand, autophagy inducers can rescue autophagy block and cell survival in Npc1 cells, whilst in Atg5 KO cells true autophagy inducers are not able to rescue autophagy or cell death. This provides us with an opportunity for a unique and rapid high throughput cell death-based screening system. Compounds that are capable of activating autophagy and overriding the autophagy block in Npc1 KO cells rescue cell death, whilst their dependence on functional autophagy is indicated by the lack of effect in Atg5 KO cells.

Additionally, we generated and optimised for HTS wild type or Npc1 KO MEFs with an inducible tet-on-tet-off expression of a luciferase-tagged autophagy flux reporter p62. As a proof of principle, we performed a screen using a library of FDA-approved drugs, provided by the Newcastle High Throughput Facility. The screen produced 12 small molecules previously not known as autophagy inducers that effectively activated autophagy flux. Finally, we generated and optimised wild type or Npc1 KO cells stably expressing “traffic-light” EGFP-RFP-LC3 for high throughput high content screening. Both platforms will be used for secondary/tertiary screening purposes.

We propose to initiate a drug discovery programme with the aim of identifying novel bioactive autophagy inducers.

Team

Viktor Korolchuk (VK), cell biology, Newcastle University, UK;
Jóhannes Reynisson (JR), drug discovery, Keele University, UK; and
Konstantin Volcho (KPV), organic and medicinal chemistry, Novosibirsk Institute of Organic Chemistry, Russian Academy of Sciences.

Next Steps

KVP lab collected 1000+ compounds initially isolated from rare plant and animal species from northern Russia and have a unique expertise in the synthesis of these compounds and their structural derivatives.

This is a virgin collection that has never been tested for its effect on autophagy and, combined with the natural occurrence of these molecules and therefore bioavailability, it increases the chances of successful hit identification. In addition to chemical synthesis, KVP also brings in vivo testing capacity, subject to initial identification of drug leads as outlined below.

We will initially test a small (~200) collection of compounds which are readily available and represent a diverse chemical variety present in the library. The hits from the initial screen will be processed through secondary/tertiary readouts. Lead molecules will be identified by testing structurally similar derivatives of the hits identified in the KVP collection by our long-term collaborator JR and synthesised by KVP staff for structural verification, followed by validation of their effect on autophagy in several standard assays building a preliminary structure activity relationship (SAR).

Our follow up aim will be to establish the specificity of these and other small molecules from the screens, identify their cellular targets (though Samsara platform), and characterise their mechanism of action in autophagy. We will also investigate the potential of these molecules to alleviate cellular defects caused by lysosomal dysfunction (e.g. mitochondrial deficit, DNA damage, increased sensitivity to stress and cell death) using human fibroblasts and neurons. In parallel, we will test a focused collections of small molecules based on the structure of our lead compounds to establish a robust SAR for future translation into preclinical models.

Budget

Identification of lead compounds:

1. Screen a diverse library of naturally occurring bioactive compounds (~200) in cell survival assays (Atg5 vs Npc1 KO) 🡪 dose response effect (VK) (£5,000, 2 months including optimisation and set up)

2. Hits selection based on their chemical diversity, chemical tractability, and physicochemical parameters (JR) (£2,000, 1 month)

3. Hit verification screening 🡪 Orthogonal assays (Luc-p62 clearance, traffic light LC3) (VK) (£3,000, 2 months)

4. In parallel (2 months):

   • Synthesis of derivatives for 3-5 hit series, ~12 each (JR, KPV) (£10,000);
   • Additional autophagy assays (autophagic cargo degradation; flux assays; imaging-based determination of autophagy induction; testing an involvement of known signalling pathways) (VK) (£5,000)

5. Lead series determined by screening (VK) (£2,000, 2 months)

6. In parallel (2 months):

   • Second round of synthesis based on lead series ~12 derivatives (KPV, JR) (£3,000);
   • Testing the ability of lead compounds to alleviate cellular defects caused by lysosomal dysfunction (e.g. mitochondrial deficit, DNA damage, increased sensitivity to stress and cell death) (VK) (£5,000);
   • Determination of biological target (Samsara)

7. Screening of derivatives, SAR determination, identification of drug leads (KPV, JR, VK) (£3,000, 1 month)

Total: 12-month postdoc + running costs - £80,000

Future work subject to successful screening:

8. ADMET, DMPK profile determined in mouse models, (KPV) (Total £16,600, 4 Months)

   • Pharmacokinetics, tissue distribution, excretion (£3,300)
   • Routes of administration: PO, IV – (£3,300)
   • Preliminary tox studies (dose-range finding, MTD) (£10,000)

9. IP sought for drug candidate(s) 🡪 patent

TTO overhead (20-60%) is not included in the current budget and might increase the ticket size up to $250000

Contingency:

10. Back up screen as required (1000+ natural bioactive compounds can be synthesised and screened) (KPV and VK)

Thanks for the great proposal and writeup!! Wonder if it could be valuable to have a clear sense what the conviction is of the evaluators… could something like “strong yes, yes, neutral, no” with numbers of evaluators attached to it be valuable?

One additional important point to make - we have not taken into account the overhead that will be charged by the TTO (anywhere from 20-60%), thus the ticket size will be substantially larger than budgeted above (closer to $200k).

I’ve made some edits to answer the comments above. In two days this should be ready to go on-chain

The proposal should probably go on chain with $250,000 as the ticket size. We are just finalising the terms and costing with the TTO, and it will likely be very close to $250,000 in total. I have edited the proposal to reflect this update.

The final costing, including research cost, overheads (university, Molecule, legal), and IP-NFT artwork come to $285,000 USD in total. This is $35,000 additional over what passed on chain, which falls beneath the threshold for requiring a vote. The proposal - as you can see above - was moved on-chain before the final costing was received by the university, which created this issue.

In the future, we can take two paths for avoiding this issue:

1. Waiting for a final costing from the university to put proposals on-chain. This has the downside of making us move slowly, but having an exact idea of the final cost.

2. Have a larger range in the proposal to be flexible and move quickly.

Thanks for the transparency, Tyler. I will definitely have this in consideration for the next proposal.

I would prefer the second option: trying to get a ticket range informative enough for the community to vote but broad enough to give room for negotiations with the TTOs. Waiting to get a final cost before even knowing if the community wants VitaDAO to fund the project could waste a lot of negotiation time. I would rather try to check the pulse of the community as early as possible before putting that much work into a project. However, I also understand that the final cost can be a huge factor to decide if a project is worth funding or not, so I’m really looking forward to hear how the community feels about it.