From SBS' President
Transitions:
SBS Forges Ahead
By Al Kolb
As is the tradition in SBS, the annual meeting is the time when the presidency
of the society changes hands. In September, Dejan Bojanic stepped down as President
and will now serve as Past President. He has done a great service to the society
and helped us to implement changes that will have a long lasting and positive
impact. I look forward to working with Dejan over my tenure as President and
drawing on his experience and expertise. At the same time, Ricardo Macarron became
President-elect and will work with us and the Board of Directors to guide SBS
into the future. A final thank you goes out to Sitta Sittampalam who returns
to civilian life after his tenure as Past President.
Society Name Change
Before Dejan stepped down, he opened the 11th Annual SBS Conference and Exhibition
of the Society for Biomolecular Screening in Geneva, Switzerland. At this opening,
he announced the results of the vote by the membership in favor of changing
the name to the Society for Biomolecular Sciences. We are still SBS, but the
name change reflects how the society has already adjusted to the changing world
of drug discovery. Many of the process controls, assay technologies, readers,
liquid handling and automation that were implemented and optimized in HTS labs
have been adapted by other areas of drug discovery. Target identification and
validation, lead optimization, profiling, ADME and toxicology, along with HTS,
have all become a part of the drug-discovery continuum. This has led to the
development of a more streamlined and efficient drug-discovery process. Since
the skills and technologies learned in HTS are now used in so many other areas
of drug discovery, in universities and government labs as well as pharmaceutical
companies, it is appropriate to include scientists working in these areas in
SBS, but still continue a strong, core program for our HTS members.
The name change discussion has been ongoing within the Board of Directors
for almost five years. As a way to test the opinions of the members, an outside
marketing firm was contracted to conduct a survey and phone interviews with
a number of members that would represent a statistically significant sample.
The results supported a name change and the Board felt it was in the best interest
for the future of SBS to present the change to the membership for a vote. The
vote was conducted by a firm specializing in on-line voting so that no one
associated with SBS was involved. The results of the vote showed that a majority
of the members approved the name change: 56% voted for in favor of the change
and 44% were not in favor; 23% of the eligible voters cast ballots, which closely
matches the 22% who voted for Board members in 2005.
Some of the members who were not in favor of the change expressed concern
that SBS is moving away from its core constituency and founding members. We
want to assure all our members that including related disciplines in drug discovery
does not mean that we will abandon our core. We have always been a close-knit
society with a common interest in improving the drug- discovery process, better
understanding the biology of disease and finding safer, more effective lead
compounds. This will not change.
Members who are concerned will see that the Journal for Biomolecular Screening
(which will not change its name) will still have the same quality articles
on HTS-related subjects, and our annual meeting will still have core sessions
directly related to HTS. However, you will also see us expand into other areas
such as biomarkers and target biology. Both these sessions were held at our
annual conference in Geneva and had significant attendance. This indicates
the diverse interests of our members.
Just as ADMET was once a downstream process not associated with HTS, it is
now often done by HTS groups and it has become an essential part of the annual
conference. The Board is working with the conference committee to ensure that
the annual conference will continue to have sessions on core topics. These
core topics include such areas as new technology (assay comparisons, automation,
screening advances), target biology, ADMET, compound management (library design
and compound logistics) and cheminformatics. Ultimately, it is the feedback
from the members that determines the content of the conference and its success,
so your suggestions are important.
I strongly believe that adjusting to the changes that are occurring in the
organization and the function of early drug discovery will allow SBS to remain
relevant to current members and attract new members from related fields. This
will bring in new ideas, keep us better informed and help us to improve drug
discovery.
Extending Our Reach
While I hope that I have been able to reassure our members about the name change
and the importance of HTS, there are also challenges and opportunities that
we face. The activities and programs we offer are designed primarily to help
our members through education and networking. It is our responsibility to make
SBS programs accessible to as many members as possible. The Journal, newsletter
and web seminars give people in almost any location a chance to be a part of
SBS.
While the annual conference is by far the best opportunity to exchange ideas
with colleagues, learn from experts and view the latest technology and products,
it has limits in the audience it can reach. That is why SBS is working to establish
a program of regional meetings in the US, Europe and other locations. We have
had successful regional meetings in the San Francisco area, in Madrid, Spain
with the Spanish Society for Biotechnology (SEBIOT), and in association with
Harvard University in Cambridge, Massachusetts. We would like to increase the
number of these regional meetings and include more international locations.
Thirty percent of SBS members come from outside the US, primarily from Europe.
We would like to increase our worldwide membership, and a program of regional
meetings would not only benefit current members, but also introduce SBS to
potential members. In addition to Europe, we would like to organize and participate
in meetings in other regions with strong pharmaceutical research. This would
include India, Japan, China, Taiwan and Australia. Learning more about drug
discovery in other parts of the world will improve the exchange of ideas and
strengthen the society. This is an ambitious undertaking and will take some
time to properly staff, manage and organize. However, a strong program of regional
meetings will complement the annual conference and give SBS a more global presence.
We will have to rely heavily on our members and other organizations in these
countries to help arrange conferences. Volunteers are always welcome.
The field of HTS, early drug discovery and pharmaceutical research have changed
significantly over the 11 years since the beginning of SBS and if anything,
the change is accelerating. As a society, we have to remain relevant and vibrant
by adjusting to accommodate new members while continuing to support our loyal,
core members.
I welcome the challenges that the next year will present and welcome input
from our members on how we can make SBS a better organization. You can take
an active part in your society by sending your ideas and comments to SBS at
email@sbsonline.org
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SBS/NIH Connections
Behind the Scenes at the NIH Molecular Libraries Small Molecule Repository
By Douglas Livingston & Tim Lease
Discovery Partners International
The Molecular Libraries Small Molecule Repository (MLSMR) is a central component
of the NIH Roadmap Molecular Libraries Initiative (MLI; see interview with
Chris Austin in the pre-conference issue of SBS News). Over the next decade,
the MLSMR is intended to host up to a million compounds comprising the central screening
compound collection of the MLI. It is responsible for compound acquisition,
curation, and the distribution of formatted samples to specific centers established
within the MLI. It is not feasible within the current budget to distribute samples
of the repository screening collection more broadly to the research community
outside the scope of the MLI; however, all of the compounds in the collection are being
registered in the publicly accessible database PubChem (http://pubchem.ncbi.nlm.nih.gov),
including searchable structures and other relevant information about each compound,
and all screening data as it is generated by the MLI (search on “SMR” in
PubChem to extract the current set of Repository compounds).
MLSCN Ups the Ante
The Repository is administered under contract by our company, Discovery Partners
International (DPI; www.discoverypartners.com), and is physically located in
a newly renovated 4,000 square foot facility at the DPI site in South San Francisco.
During the first year of the project (beginning August 2004), we were fortunate
to work closely with the NIH Chemical Genomics Center (NCGC) staff.
More recently, our scope of interaction took a quantum leap in complexity
with the completion of the Molecular Libraries Screening Center Network (MLSCN)
in June, when three-year grants were awarded by NIH to establish extramural
screening centers at nine academic institutions spanning the continental US
(www.sbsonline.org/nih/archi/2005.06.php for more information).
Frequently controversial, often misunderstood, the MLSCN is the publicly accessible
screening consortium of the MLI, set up specifically to identify innovative
chemical tools that will enable the next era of fundamental medical, biological
and chemical genomics discovery. None of these activities are intended to capture
or compromise intellectual property in a manner that would harm pharma or other
private sector interests. The unexpected amount of concern and wary interest
that has been expressed to date is not surprising in hindsight; the 10 (including
NCGC) centers of the MLSCN now collectively represent an impressive arsenal
of bioassay technologies. And to us, they collectively represent a daunting
appetite for plates of screening samples that need to be supplied in a timely
manner across a range of capacities and formats.
Two key aspects of the MLSMR project are unique. First, the components of
the MLI are typically distributed across extramural centers or are a combined
effort among multiple NIH Institutes. Because of the advantages in centralizing
the stewardship of a large compound collection, the MLSMR is an exception.
For analogous reasons, PubChem has also become an intramural nexus of the MLI.
The practical consequence for us is that an unusually large number of interactions
need to be supported, particularly during the initial phases. This will continue
to increase as more screens are implemented, and the number of compound suppliers
expands.
Second, the MLSMR is funded under a contract, not a grant; the latter is by
far the more common extramural funding instrument used by NIH. DPI is thus
obligated to specific deliverables and must follow the rules required of any
US Government contractor. It also means that vendors of compounds and equipment
must become subcontractors to the DPI contract, with much the same obligations
as DPI. Many of the available compounds must be sourced from companies based
in former Eastern Bloc nations. Establishing these companies as US Government
subcontractors for the first time has been an interesting, but surprisingly
straightforward process. The interest and enthusiasm of potential compound
suppliers to the project has been very high. However, establishing vendors
properly is a sequential process, determined by available resources. We encourage
everyone to update us on your offerings regularly. Given the large appetite
for diversity on this project, we expect that a large percentage of the available
vendors will be represented in the library as we move forward.
In summary, our objectives under the MLSMR contract are to identify and acquire
appropriate compounds; do quality control and store the compounds; create and
distribute compound arrays for screening; monitor compound inventory and re-supply
or re-synthesize as appropriate; implement an inventory database, interface
with PubChem, and create a public website; deliver various reports to NIH;
and interact with other components of the Molecular Libraries Roadmap Initiative.
Building the Repository
So what is the composition of the collection, and how was that determined?
Our first step was to identify the classes of compounds to put into the repository.
In part due to budget constraints, this goal is framed by what compounds we
can gather from a combination of commercial purchases and donations from government,
academic, and other sources. To jump start collection of the first 100,000
compounds, we focused on the most readily available compounds—those from
commercial suppliers. We created a database of approximately four million commercial
HTS compounds from approximately 25 international suppliers.
We grouped compounds into four categories: Specialty Sets (SS) comprising
known bioactives, drugs, toxins, and others; Natural Products (NP); Targeted
Libraries (TL), subcategorized into protease, kinase, GPCR, ion channel, and
nuclear receptor sets; and Diversity Compounds (DC) comprising compounds that
didn’t fit into the other three categories. DPI accepted TLs as advertised
by the suppliers and did not assess the validity of the suppliers’ claims.
For the first 100,000 compounds, MLSMR targeted 80,000 DC, 15,000 TL, 3,000
NP, and 2,000 SS compounds.
MLSMR selected compounds for acquisition based on multiple criteria, which
were established based on input from a panel of advisors convened by NIH. Compounds
were required to be at least 90% pure according to the suppliers (MLSMR tested
the purity of each compound when received - vide infra) and needed to be available
in 10 mg quantity. MLSMR further filtered DC and TL compounds to meet the Lipinski
Rule of Five and calculated water solubility of at least 20 micrograms/mL.
Since the MLI is geared toward discovery of molecular probes and not drugs,
these requirements were simplifying assumptions for the first 100,000 and weren’t
intended for the entire collection. Any bias introduced to the collection by
these filters will be corrected in later stages of compound collection. We
also filtered DC and TL compounds for chemical substructures representing reactive
functional groups or moieties known to interfere with HTS.
Finally, MLSMR used Daylight fingerprints to select diverse sets from the
DC and TL compounds passing the physicochemical and excluded functionality
filters. We clustered each diverse compound with up to four nearest neighbors
of between 85% and 99% Tanimoto similarity. MLSMR collected these micro-clusters
to provide instant structure activity relationship (SAR) data for screening
hits. Having near neighbors was optional for the first 100,000 compounds and
only 34% of the diverse compounds had at least one close analog as defined.
Based on input from the screening centers, greater emphasis will be placed
on selecting these micro-clusters in future acquisitions.
Once we identified—and NIH approved—the desired compounds, MLSMR
commenced sample acquisition. In our standard process, we send bar-coded, pre-tared
4 mL glass vials to suppliers, who fill the vials and return them to MLSMR.
Of 125,000 selected compounds, 90,000 were available in the desired 10 mg amount.
We process received compounds in a standard, high-throughput quality control
regimen that checks the weight, solubility, identity, and purity of the samples.
MLSMR first checks the sample weight to ensure we receive minimum amount required
from suppliers; then, it dissolves the samples in a volatile solvent mixture,
90:10 chloroform/methanol, and removes aliquots LC-MS analysis and our DMSO
Working Store solution. We completely remove the volatile solvent from soluble
samples, along with the LC-MS and Working Store aliquots; insoluble samples
are rejected.
We check sample identity and purity by LC-MS using two Waters eight-channel
MUX LC-MS instruments with combined capacity to analyze one million samples
per year under a variety of conditions. MLSMR accepts samples where the molecular
ion is identified and Area Under the Curve (AUC) is at least 90% by Evaporative
Light Scattering (ELS) or UV (at 214 nm) detection.
Of 90,000 samples collected by MLSMR to date, 67,000 passed all the QC criteria
and are available for distribution to the MLSCN screening centers. Samples
that pass QC are stored in automated storage equipment for fast retrieval.
We have a three-tier storage system. The bulk sample is stored in what we call
our Long Term Store: the sample is neat at -20 °C under N2 in glass screw
cap vial. The long term store samples are designed to be stored for five to
ten years. Our long term store vials are stored in a DPI Universal Store, an
automated sample storage and retrieval system. The universal store will store
up to 500,000 of the 4 mL vials, and can load and retrieve up to 60,000 vials
in eight hours.
An approximately 3 micromole sample of each compound is contained in a working
store: a 10 mM DMSO solution in a 0.5 mL polypropylene tube. We use aliquots
from the working store samples to create the microtiter plates shipped to the
MLSCN screening centers. DMSO solutions of the compounds are always stored
and handled under N2 atmosphere to prevent water absorption. We’ve validated
that our process minimizes water absorption and haven’t observed compound
precipitation from the DMSO solutions.
Distributing Compounds
The current compound quota is 450 nanomoles per screening center per year,
not including material for hit follow up. MLSMR delivers the full repository
collection for standard screening to each center up to two times per year.
To date, MLSMR has distributed starter sets of approximately 3,000 compounds
to nine of the 10 MLSCN centers, including two locations for one center. The
current 67,000 compound set is available to the centers and we’ve begun
delivering the full set upon request.
The MLSMR project requires extensive data tracking. DPI created ComIT (Compound
Inventory Tracking), an Oracle based application to track, manage, and report
all sample operations from ordering from our suppliers through shipment to
the screening centers. ComIT is a customization of CambridgeSoft’s Inventory
Enterprise application that coordinates what physically happens in the repository
and communicates it to users inside and outside DPI. Repository workers access
the application by a standard web browser interface and use ComIT to automatically
guide and record their work.
MLSMR deposits the structures of compounds accepted into the repository into
PubChem. The MLSCN screening centers will link to these substances when depositing
their HTS data with PubChem. In tandem, DPI is building a public website specifically
oriented to MLSMR activities that includes descriptions of the repository and
its compounds. Eventually, the MLSCN screening centers will use the website
to order their compounds and the public will be able to search and browse all
compounds available in the repository.
In closing, we would like to share an observation. We opened this article
by giving a sense of the diversity of opinion that has existed regarding the
nature of this program. Admittedly, we at first found this wide diversity of
opinions to be disconcerting. But over time, we have learned to see the juxtaposition
of such diverse opinions as a core strength of the NIH culture, and now fully
appreciate NIH’s impressive ability to bring together passionate individuals
with widely differing opinions in order to extract the best thinking of our
nation’s scientists. Consensus is not a necessary outcome.
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Advancing The Science of Drug Discovery
In This Issue:
Offers Scientists "Limitless Opportunities"
