Adding Precision Tools to the Plant Biologists' Toolbox with Chemical Genomics

doi:10.1104/pp.104.900155

Adding Precision Tools to the Plant Biologists' Toolbox with Chemical Genomics

Natasha Raikhel^* and Michael Pirrung

Botany and Plant Sciences Department (N.R.), Chemistry Department (M.P.), and Center for Plant Cell Biology (N.R., M.P.), University of California, Riverside, California 92521

The scope of our knowledge regarding plant genetic mechanismsand gene functions is rapidly evolving and expanding. This isprimarily due to the availability of genetic and genomic methodsfor investigating model species, such as Arabidopsis (Arabidopsisthaliana). To fuel future advances, current gene-based methodsmust be complemented by innovative interdisciplinary approachesthat are broadly applicable to dynamic and complex biologicalprocesses and functional genomics analyses. We believe thatthe use of diverse chemicals to interrogate molecular processesprovides a novel avenue for the rapid and effective dissectionof biological mechanisms and gene networks in ways not feasiblewith mutation-based approaches. By facilitating the identificationof new pathways and networks, this powerful technology, calledchemical genomics, overcomes important gaps in ongoing functionalgenomics efforts in plants and allows for the eventual developmentof a framework for predictive modeling.

The chemical genomics approach uses small molecules to modifyor disrupt the functions of specific genes/proteins (Stockwell,2000; Dobson, 2004; Lipinski and Hopkins, 2004), in contrastto classic genetics, in which mutations disrupt gene function.The underlying concept is that the functions of most proteinscan be altered by the binding of a chemical, which can be foundby screening large libraries for compounds that specificallyaffect a measurable process. There are four major aspects tochemical genomics: (1) library assembly/synthesis, or the creationof chemically diverse libraries of compounds; (2) screening,or the identification of compounds that affect a biologicalprocess of interest; (3) target identification, or the discoveryof the protein targets of active compounds; and (4) target functionand network discovery, or the use of the compounds to understandbiological processes. It is usually necessary to screen a largenumber of compounds to find one or a few of sufficient specificityand efficacy to be useful, analogous to genetically screeningfor mutations causing a specific phenotype. However, the chemicalgenomics approach can address loss-of-function lethality andgene redundancy and allow instantaneous, reversible, tunable,and conditional control of a phenotype, providing many advantagesover traditional genetic approaches. Well-characterized bioactivechemicals and their targets identified in Arabidopsis can beused in non-model species to improve agronomic traits and increasecrop value.

Bioactive chemicals have a long history of helping plant physiologistsunravel mechanisms, including those involving inhibitors ofGA biosynthesis, inhibitors of ethylene action, inhibitors ofauxin transport, cytoskeleton-disrupting drugs, and inhibitorsof GDP-GTP exchange proteins, just to name a few. However, thisapproach has also met with strong criticism due to the complexitiesassociated with understanding the action mode of compounds atthe molecular level. This is one reason why drug companies mustadvertise the side effects of the drugs they sell. What hasmotivated biologists to revisit their interest in small molecules?

While a little more than 10 million pure compounds are knownin chemical literature, the potential chemical diversity (definedas the number of unique chemical structures) of compounds composedof carbon, hydrogen, nitrogen, oxygen, sulfur, phosphorous,and the halogens (the organic chemist's periodic table) of molecularweight <1,000 likely exceeds 10⁶⁰. The compounds that havethus far been tested for effects on plants are therefore onlya minute fraction of the structural possibilities. The developmentof combinatorial and automated techniques for synthesizing novelcompounds brought forth significant enhancement in the productivityof chemists and makes the likelihood of synthesizing molecularlibraries that are representative of "chemical space" much greater.These advances in technology allow a systematic analysis ofthese chemicals. A more systematic approach means that we discoverchemicals that specifically disrupt a process or the functionof a protein. Once these chemicals are identified, we can combinetheir use with genetic screens to identify genes involved inthe same process. The use of unbiased libraries of diverse smallmolecules will allow plant biologists to discover numerous newbioactive molecules valuable for studying the function of uncharacterizedplant genes. Importantly, when combined with Arabidopsis functionalgenomics, chemical genomics is powerful for the effective andefficient analysis of regulatory networks underlying a specificprocess.

Chemical genomics technologies have been used by industry fora long time. The only academic institutions devoted to thisapproach with a focus on mammalian cells and microorganismsare the Broad Chemical Biology Platform (former Institute forChemical Biology) of Harvard University and the National Institutesof Health Chemical Genomics Center (Dobson, 2004). Chemicalgenetics approaches have been used to dissect pathways in single-celledsystems, including bacteria, yeast, and mammalian cell culturesand in Caenorhabditis elegans and zebrafish. Several studieshave shown that identified chemicals can exhibit extremely highspecificity toward target proteins. The major challenge in mammaliansystems is the identification of target proteins because ofthe lack of an efficient molecular genetic/genomic approach(Stockwell, 2000). This problem has been acknowledged by recentapproaches to develop knockout collections in mice (Austin etal., 2004). Several recent reports in the field of plant biology,however, have demonstrated the feasibility of chemical genomicsin Arabidopsis (Armstrong et al., 2004; Zouhar et al., 2004;Surpin et al., 2005), but the approach has not yet been widelyaccepted by plant biologists.

We argue that chemical genomics has several major advantageswhen integrated with Arabidopsis genomics/proteomics tools,including the capabilities to: (1) effectively dissect a complexgene network affected by chemicals of interest; (2) rapidlyidentify their gene targets; and (3) efficiently investigatetheir mode of action. The reference plant Arabidopsis with itssmall body size and high seed yield is ideal for chemical screensat various biological levels ranging from subcellular to thewhole organism. Arabidopsis offers many unique genetic/genomictools, including a completely sequenced genome (ArabidopsisGenome Initiative, 2000), whole-genome microarrays, a largecollection of knockout and activation-tagged mutations, a richarray of mutants, and the ease of cloning a gene by map-basedcloning aided by DNA microarrays. Arabidopsis was invaluablefor the identification of receptors for brassinosteroids (Wanget al., 2001) and ethylene (Schaller and Bleecker, 1995), justto name a couple.

Critical to the chemical genomics approach is the ability toscreen for mutants resistant or hypersensitive to bioactivechemicals and to identify responsible genes using genomics-basedmethods. Mutations conferring resistance/hypersensitivity caneither affect the target of the chemical, or upstream and downstreamcomponents of its target. Once responsible genes are cloned,cognate target proteins may be identified by further studies,such as chemical binding assays. Importantly, mutations in acomponent upstream/downstream of the target protein will notonly give insights into the function of target genes but alsoprovide a new high-throughput method for identifying new genesin the corresponding network. In other words, chemical genomicswill enhance the power of existing genomic tools including thelarge collections of T-DNA insertion lines, from which we canrecover mutants with altered chemical sensitivity that otherwisemay not exhibit a phenotype (Blackwell and Zhao, 2003). Thus,the integration of chemical genomics with Arabidopsis genomicsprovides a strategic advantage and a powerful high-throughputapproach for gene network discovery, target identification,and mode-of-action studies.

Of course, it is necessary to use chemical genomics with caution,and the tool has its own limitations. For example, the specificityof the selected compounds needs to be addressed, and possibleuptake and metabolism of the compounds may affect the discoveryand analysis of bioactive compounds. Consideration of knownmechanisms of metabolism suggests strategies for the designof metabolism-resistant small molecule libraries. For example,fluorinated or cyclopropyl compounds that are resistant to cytochromeP450 oxidation are well known. Such oxidation-resistant groupingscan be used in the construction of chemical libraries to preventmetabolism. This will help assure that mutants that are resistantto a "hit" chemical have modified targets (or at least modifiedproteins in the same pathway). As with any new technology, chemicalgenomics has its pros and cons. However, we believe that chemicalgenomics offers a strategy to extend the applicability of functionalgenomics in plants by addressing issues of overlapping genefunction in gene families, lethal loci, and control of dosage-and tissue/development-specific applications.

FOOTNOTES

www.plantphysiol.org/cgi/doi/10.1104/pp.104.900155.

^{^*} Corresponding author; e-mail nraikhel{at}ucr.edu; fax 951–827–2155.

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