So Im a small-molecule drug discovery person at heart, since I started out as a synthetic organic chemist. Talking about vaccines and antibodies nonstop is a bit of a strain, then, because immunology is full of stuff thats rather far removed from good ol small-molecule ligands. Actually immunology eventually wears out everyone. Even immunologists. It just keeps on going: detail on top of detail, layer upon layer of complex, interconnected, rococo feedback loops and backup systems, repurposed evolutionary holdovers, insanely subdivided cell lineages, all the rest of it.
But in the end, even a medicinal chemist starts to feel at home in some parts of it. Because one of the key events in the adaptive immune system is exactly like one of the key events in so many small-molecule drug research programs: high-throughput screening. I know that I have a lot of people reading this who have never done any such thing, so its worth some explanation. Now, in traditional med-chem and its allied fields, HTS has been a way of life for around 30 years now (before that it was low-throughput screening!) Its had a lot of refinements and extensions, but the fundamental process has not changed one bit: round up some of your biological target (an enzyme, a receptor, an interaction between two proteins, whatever youve got), and find some setup where you can get a signal when a compound does what you want to it. Do you want to set off a signal from a receptor? Keep two proteins from coming together? Gum up the works of some enzyme? Work up some assay system where when that desired event happens, you get a signal that come up out of the noise.
It could be (and often is) a flash of fluorescence at a particular wavelength. That idea has had plenty of changes rung on it maybe youre looking at two wavelengths at the same time and checking the ratio between them. Or you can set things up where its the polarization of that fluorescent light thats telling you something. Maybe youre running things in a way where the fluorescence is already going on and your desired stuff will shut it off. You can have fluorescent probe compounds; there are whole careers involved with those things. Then there are of course fluorescent proteins (like the famous Green Fluorescent Protein), and listing the ways that those are used in assays would take us the rest of the week. Theres are physical phenomena that will allow fluorescence to be set off only when two suitable species are close enough together in space, and as you can imagine, these have been turned into workhorse assays.
Luminescence can be used in similar ways. The enzyme luciferase has been exploited six ways from Sunday, with a long list of variations. Any good screening lab has a list of their compounds that have been shown to directly interfere with the enzyme (and can thus hose up your data). We love luciferase so much that we use both the firefly kind and one from a deep-sea critter called a sea pansy because they come in both green and red versions (and sometimes you use both of those at the same time, too). That same sort of only when they come close together trick can be worked with luminescence, too. No. there are all sorts of tricks you can play with funny wavelengths of colorful light, and all sorts of interesting ways you can set up assays to emit them.
But it doesnt have to be light. A classic way to do receptor assays (and others) is to have a radioactive compound already stuck to your target. You add some of your test substance and see if it kicks any of the hot stuff off, which you read off after a filtration step: the more radioactive your filtrate, the better your compound bound to the target. You can mix radioactivity and a light-driven readout, with a scintillation proximity assay: a radioligand that gives off a beta-particle lights things up only when its next to your target, and not under other conditions.
No matter how you run any of these, the idea is to get such an assay set up so that theres a high signal-to-noise, low chances for false positives and false negatives, no need for too many picky dispensing or mixing steps to get it running, and (especially) the ability to run at the smallest scale you can handle. I well recall when doing such things in assay plates with 8 wells by 12 (96 total) was considered kind of high-tech, but for a long time now any assay that cant be shrunk down to 384 wells (1624) or 1536 (3248) has been greeted with a weary sigh and a roll of the eyes. There are legions of commercial assay kits and associated dispensers, plate-handling robots, and plate-reading machines that will assist you in getting all this going.
You want this miniaturization, of course, because you want to put the HT in the HTS. A full-deck screen at a big drug company can be a few million compounds if you pull out all the stops (which we dont so often any more, to be honest), and doing that 96 wells at a time will take you a while. Especially when you consider controls and duplicates, and youd better if you dont want to seriously waste your time. No, if youre going to screen a really impressive set of compounds, youre going to need all the help you can get. The latter 1990s and early 2000s in the drug business was a period when the high-throughput screeners and the combinatorial chemists tried to outdo each other
And heres where we get back to coronaviruses, antibodies, and vaccines. Because high-throughput screening is what goes on in your bloodstream constantly, as your adaptive immune system watches for pathogens. Everyone carries around a huge variety of different antibodies, all of which fit into some basic structural templates. No one is quite sure just how many different antibodies a person has, actually, because a real count is just an overwhelming task: the usual guesses are in the tens of billions, hundreds of billions, maybe a trillion different ones, which is a hard number to grasp. Imagine a company with a million compounds in its screening deck (OK), and then try to picture a million such companies (nope, not happening). And it might be a lot more incomprehensible than that the first link in this paragraph will take you to a paper that estimates that the available diversity for circulating antibodies is on the order of 10 to the 18th, and whats yet another factor of a million between friends? Given the combinatorial possibilities, it is beyond certain that no two humans have ever had the same repertoire of antibodies, and that no two humans ever will.
These things are floating around in your blood and being displayed on the surface of your various B cells (a mere hundred thousand or so per B cell), just waiting to see if there might someday be something that they bind to. Theyre just like a compound collection in a drug company, actually, except theyre not being stored in separate vials or wells, but are rather dumped all together in your bloodstream. And the assay conditions have been long worked out by evolution, with a huge signal/noise: activation of complement or of the various types of effector cells that respond so dramatically to the presence of antibodies bound to an antigen target.
Theres actually a screening method used in drug discovery thats broadly similar to this: DNA-encoded libraries. Thats where you build up a huge set of small molecules, each of which has its own DNA bar code attached to it. You screen these all at once, too you can hold up a small plastic Eppendorf vial that has (easily) tens of millions of different compounds in it, each with its own DNA identifier. You run the assay in a way that you pan for the potent binders, washing the less potent ones out of the system. Then after you finally knock the strong binders off with stronger conditions, you amplify and sequence their DNA barcode regions and get a reading of what small-molecule structures they must have been. That makes it sound relatively straightforward, but doing this right takes a good deal of care and a lot of data analysis of the hits at the end.
But you can see how it works in a roughly similar fashion to the way native antibodies work in our own bloodstreams. You start with a large variety of compounds, all mixed together, and you try them against a given target. When one of them binds strongly, you use some sort of amplification to pick out this rare event which is present in extremely small concentration. With DNA-encoded libraries, its getting rid of all the weaker binders by washing them off, and using PCR to make far more copies of the DNA sequences you have left. In the immune system, the amplification is built into the cellular responses, which propagate strongly through the immune system and set off further responses in turn.
The immune system is a lot more impressive, of course. Its had a long time to get better, under constant whole-organism threats of illness and death and subsequent inability to reproduce. The screening collection in any single humans bloodstream is far larger than any human efforts have ever reached, so the amplification of any given binding signal has to be a lot more robust. Thats been under serious selection pressure as well, of course: if we pick the wrong compound in a screening effort we will waste time and money, but if the immune system picks the wrong antigen to go off on, it can start attacking your own bodys tissues and kill you. The amount of infrastructure thats been built up over the millennia to avoid that is pretty intimidating all by itself.
Note that we wouldnt even be able to do the DEL trick without piggybacking on all that evolutionary work, either. The ligase enzymes that allow us to build up the DNA barcodes and the PCR that lets us amplify the DNA at the end yeah, we stole all that and repurposed it, and theres no way that you could ever get things to work without them. But its just like the fluorescent proteins mentioned above molecular biology and chemical biology depend on being able to repurpose the amazing array of tools found in living cells. Weve added plenty of our own technologies as well. No living organism does anything like electrospray mass spectrometry, Frster resonance energy transfer, NMR, surface plasmon resonance or the like. But combining what weve learned of chemistry and physics with what evolution has developed, you can run some pretty fancy systems, which are getting fancier all the time.
But for sheer library size and ability to pick out hits, nothing we humans have been able to put together rivals the adaptive immune system. Perhaps thats been one minor side effect of the pandemic: people who have taken the time to learn a bit about immunology can only come away with a sense of awe when they start to see the huge panorama of whats been going on inside their bodies for every second of their lives.
Read more:
Screening, Within and Without | In the Pipeline - Science Magazine
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