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This is the place where we will describe some of the outcomes and results of your folding work, provide a glimpse of future challenges and developments, and in general give you a better sense of where we are and where foldit hopes to go in the future.

The story of a Foldit design

As discussed in previous blog posts, some Foldit player solutions from design puzzles are chosen for synthesis in the Baker Lab. One design in particular, from Puzzle 854, has recently yielded some promising results in the wet lab. Below, we follow this design's journey from video game to test tube:

1. Once we select a design to be synthesized in the lab, we extract the amino acid sequence from the design and reverse transcribe this into a sequence of DNA bases (i.e. a gene), adding a special tag that will come in handy later.

2. We order this gene as a DNA molecule from a gene synthesis company, and splice the gene into a larger, circular piece of DNA called a plasmid. The plasmid now containing our gene is inserted into E. coli bacteria, which we allow to grow and reproduce in an incubator. These bacteria will transcribe and translate our gene as if it were one of their own, producing our design as a polypeptide chain; if the protein design is good, the polypeptide chain will naturally fold up into the design structure.

3. Once the bacteria have grown to saturation and produced a large amount of our protein, we break open the bacteria cells and separate our protein from the other bits of E. coli using the special tag we added in step 1. At this stage, we can see whether the bacteria were able to produce our protein and whether the protein is soluble. Unstructured proteins will usually be degraded by the E. coli or otherwise form insoluble aggregates.


SDS-PAGE. A mixed protein sample (stained blue) is passed through a polyacrylamide gel from top to bottom, such that smaller proteins travel faster through the gel. Here, three samples are shown: all soluble proteins from a bacterial cell (left), proteins lacking the special tag we added in step 1 (middle), and proteins with the special tag (right). Although the first two samples have many bands (different proteins) spread across the length of the gel, the sample on the right is dominated by a single large blot (our protein) near the bottom of the gel.

4. We use size-exclusion chromatography (SEC), which separates proteins based on their size, to get rid of other protein impurities. This step also gives us information about the oligomeric state of our protein (unstable proteins with exposed hydrophobic residues tend to self-associate into oligomers). Structured monomers will behave differently on the column than oligomers or unstructured aggregates.


SEC Trace. Proteins are passed through a matrix such that larger proteins travel faster through the matrix and are collected sooner (at the left end of the x-axis); absorbance of UV light is used to measure the protein concentration (y-axis) of samples as they are collected. You can see that in the case of our protein, this step was hardly necessary because the protein is unusually pure, evidenced by a single dominant peak at 14 mL. Furthermore, the placement of the peak at 14 mL corresponds precisely to the expected size of the design, indicating the protein is monomeric.

5. After we have purified our protein, we can use circular dichroism (CD) to measure its secondary structure content. This technique measures a protein's absorption of circularly-polarized light and can tell us about the amount of α-helix or β-sheet in the protein. This measure also allows us to monitor how the protein unfolds when we raise the temperature.


Circular Dichroism. Different elements of protein structure interact differently with circularly-polarized light. At 25°C (blue trace, top) our protein shows a CD profile characteristic of a protein with a large α-helical content. At 95°C (red trace, top), the shape of the profile is less pronounced, indicating a loss of secondary structure; the secondary structure is recovered upon cooling back to 25°C (green trace, top). The bottom trace shows how the CD signal at 220 nm changes as we raise the temperature of the protein sample. The gradual, broad slope of this trace indicates noncooperative, multi-state unfolding.

The protein described above is being prepared for crystallization. If successful, we may be able to obtain a high-resolution crystal structure of the protein and make a comparison with the designed structure. Please note that we are continuing to work with other proteins that may be less well-behaved, and hope to order new designs soon!

Check out the latest design puzzle here!

( Posted by  bkoep 130 916  |  Wed, 06/18/2014 - 00:25  |  3 comments )
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Dartmouth College Scientists need your help with a Brain Cancer-related puzzle!

Having been a (novice) Foldit player myself I was aware of the potential utility of this powerful computational platform in modeling proteins even before I joined my current laboratory. When the topic of needing a structure for our protein came up in a meeting, of course Foldit was on the top of my mind. We hope that the players of Foldit can help us uncover the structural basis of Id2 activity and thereby inform the development of novel targeted therapies for Glioblastoma.

Inhibitor of DNA Binding 2 (Id2), a helix-loop-helix (HLH) protein, inhibits normal gene expression by binding and suppressing other transcription factors. Recent data from our laboratory show Id2 is a key protein in the pathogenesis of a subset of aggressive brain cancers (Glioblastoma). The structure of the HLH domain of Id2 is well characterized. However, the unknown terminal regions are very important for regulation of the protein. Having the structures for the terminal regions will help us understand how the regulation of Id2 alters its structure and function. This will help us identify regions of Id2, or proteins that
interact with Id2, which are important for degradation. We could use this knowledge to develop drugs that promote the degradation of Id2 to treat Glioblastoma.

Try out our Brain Cancer-Related Phosphorylated Id2 puzzle here. Thanks!

( Posted by cymbal_king 130 1890  |  Thu, 05/29/2014 - 16:06  |  1 comment )
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Wiggle Power Results

Earlier this year we introduced different Wiggle Powers, and a couple months ago we tried to simplify this with Auto-Wiggle Power.

We recently posted a bunch of De-novo puzzles where the "High Wiggle Power" option was disabled and hopefully the results from those puzzles will explain why we've given High Wiggle Power a time-out during CASP11.

Below are RMSD plots for De-novo Freestyle 36 puzzles 864: Low Power & 868: High Power. The green dots represent your many different Foldit predictions, and for all these RMSD plots, you want to be as close to the left as possible (an RMSD=0.0 would be a perfect match to the native).

You can see that the top-scoring Foldit solution (the lowest Rosetta energy) doesn't change much between puzzles RMSD-wise. So although the high-scoring Foldit solution for puzzle 868: High Power was 9,208 (compared to 9,098 in puzzle 864: Low Power), it is not any closer to the native.

In general (and this was the case for all the Low Power/High Power plot comparisons) although the scores were better in the High Power rounds, the models were not any more accurate. We hypothesized that this could be happening because we allowed you to load in solutions from the Low Power rounds, and therefore the High Power round was mostly "drilling" down the energy landscape of those previous models (since doing that would obviously improve the in-game score!).

This is why for 880: De-novo Freestyle 38: High Power we did not let you load in solutions from the previous Low Power round.
You can see in the plots below that this High Power round had fewer green dots, but unfortunately the results are actually much worse than the Low Power round:

On the left, 876: De-novo Freestyle 38: Low Power has a very nice plot where the top-scoring Foldit model is one of the left-most points. This is not the case on the right, where the top-scoring Foldit model from 880: De-novo Freestyle 38: High Power is much further from the native than in the Low Power round.

The exciting news, however, is that the results from the Predicted Contacts rounds have been very promising!
You can see this below for the De-novo Freestyle 37 puzzles:

On the left, the top-scoring solutions for 867: De-novo Freestyle 37: Low Power are not the left-most points on the plot (they are quite far away from the native topology) but given predicted contacts, your results on the right for 875b: De-novo Freestyle 37: Predicted Contacts look great!

The results were similar for the most recent Predicted Contacts puzzle, where we disabled High Wiggle Power and did not allow loading of solutions from 881: De-novo Freestyle 39: Low Power.

So we are looking forward to the Contact-assisted CASP11 targets, and hopefully this post explains why we'll give High Wiggle Power a rest during CASP11. The CASP season is long and busy enough that we don't want to waste your time gaining Foldit points, but not getting more accurate solutions!

Lastly, Seth and I wanted to thank all of you in the DC area who stopped by when we presented Foldit (and debuted nanocrafter) at the 3rd USA Science & Engineering Festival.
Next time we promise to give everyone a little bit more advanced notice, and we'll make sure to have a camera ready from day 1. At least we managed to snap a photo with Galaxie on the last day:

Thanks for all your hard work, everybody... and keep up the great folding!

( Posted by  beta_helix 130 3274  |  Tue, 05/13/2014 - 16:10  |  8 comments )
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Visit the Center for Game Science's Newest Projects!

Greetings Folders!

While we know you're already hard at work on the latest CASP competition, we thought we'd take a moment to talk about two new projects from the Center for Game Science: Nanocrafter and Flow Jam. These games build on what we’ve learned over the years working with you on Foldit, applying those lessons to brand new domains of scientific discovery.

Nanocrafter allows players to assemble molecular structures out of DNA. Novel designs in synthetic biology, as this new field is called, could benefit vaccines, cancer research, and more. Recently announced at the Games for Change conference at the end of April, Nanocrafter already has a rapidly growing community of builders. Help shape this new community and be sure to follow our alerts on Facebook and Twitter for the newest coverage!

Flow Jam, part of the Verigames project, is a novel approach to proving large and complex software programs free of certain errors. All newly developed software requires time-intensive testing by computers and human experts before the software can be considered reliable. If this sounds interesting to you, head over to the page and try it out, pop by the official forums, and follow our Facebook and Twitter accounts on that game for the latest news.

There’s never been a better time to contribute to scientific discovery and advancement through gaming! As veterans of Foldit we look forward to hearing your feedback on our newest efforts.

( Posted by  inkycatz 130 236  |  Mon, 05/05/2014 - 20:26  |  3 comments )
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Welcome our new Community Liaison!

Happy Monday!

To start your week off, we'd like to take a moment to introduce our new Community Liaison, Nova "inkycatz" Barlow. She'll be working on Foldit in addition to other Center for Game Science titles.

A well-established community advocate, Nova's most recent work includes Kodu Game Lab and Project Spark at Microsoft. For those fans of our IRC channel, you may have already spotted her lurking around late last week getting up to speed. She's thrilled to be joining this established community of folders and can't wait to hear your thoughts.

Feel free to say hello and offer your best folding tips!

( Posted by  inkycatz 130 236  |  Mon, 05/05/2014 - 20:13  |  3 comments )
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