INVESTIGATION Drosophila Reporter Vectors Compatible with F C31 Integrase Transgenesis Techniques and Their Use to Generate New Notch Reporter Fly Lines Ben E.Housden,KatMillen, andSarahJ.Bray1 DepartmentofPhysiology,DevelopmentandNeuroscience,UniversityofCambridge,CambridgeCB23DY,United Kingdom ABSTRACT Complexspatialandtemporalregulationofgeneactivityisfundamentaltodevelopmentand KEYWORDS homeostasis. The ability to decipher the DNA sequences that accurately coordinate gene expression is, reporterplasmids therefore,ofprimaryimportance.OnewaytoassessthefunctionsofDNAelementsentailstheirfusionto FC31integrase fluorescent reporter genes. This powerful approach makes it possible to visualize their regulatory fluorescent capabilitieswhenreintroducedintothedevelopinganimal.TransgenicstudiesinDrosophilahaverecently protein advanced with the introduction of site-specific, FC31 integrase–mediated approaches. However, most Drosophila existingDrosophilareportervectorsarenotcompatiblewiththisnewapproachandhavebecomeobsolete. Notch HerewedescribeanewseriesoffluorescentreportervectorsoptimizedforusewithFC31transgenesis.By usingthesevectorstogenerateasetofNotchreporterflylines,wedemonstratetheirefficacyinreporting thefunctionofgeneregulatoryelements. UnderstandingthemechanismsemployedbyregulatoryDNAsequen- More recently, a transformation system has been introduced cestocontrolgeneexpressionisessentialtothestudyofdevelopment which exploits the integration mechanism used by bacteriophage and disease.Tools enabling this are, therefore, ofmajor importance. FC31(Grothetal.2004).Aphageintegraseinducesrecombination Onemethodfordecipheringgenomicregulatoryinformationutilizes betweenattP(phagegenome)andattB(bacterialgenome)sequences invivoreporterassaystoassesstheactivityofputativeenhancers.For (Groth and Calos 2004; Thorpe and Smith 1998). Several groups such analysis, the DNA is subcloned adjacent to easily monitored haveestablishedtransgenicflylinescontainingattPsites(platforms) reportergenes,suchasencodingb-galactosidaseorgreenfluorescent at specific, nonmutagenic locations (Bateman et al. 2006; Bischof protein(GFP),invectorsdesignedfortransgenesis.Thisapproachhas et al. 2007; Groth et al. 2004; Markstein et al. 2008; Venken et al. been widely exploited in Drosophila, where stably inherited, single- 2006). Injection of attB-containing vectors with a source of FC31 copy transgene insertions could be generated with p-element trans- integraseresultsinintegrationofthevectorintothegenomeatthe poson-basedvectors(RubinandSpradling1982;SpradlingandRubin attPplatform. 1982). With this method, transgenes are inserted randomly in the TheFC31systemismoreefficientthanprevioustechniques,and genome, withapreferenceforpromoter regions(Bellen etal.2004). as integration occurs at specific attP sites, insertions are directly Expressionfromsuchinsertionsisofteninfluencedbythesurround- comparable and mapping is unnecessary. However, most vectors ingsequences (positioneffects),leadingtodifficultiesininterpreting forinvivoreporterassays,lackingattBsites,areincompatiblewith patternsgenerated. thismethod.TwoadaptedvectorswithattBsequenceshaverecently beenmade,butbothuseGatewaycloningandoneretainsp-element ends, precluding subsequent use of p-element mutagenesis in the Copyright©2012Housdenetal. fliesgenerated(Aertsetal.2010;Boyetal.2010).Wehavegenerated doi:10.1534/g3.111.001321 a new series of compatible vectors that contain no unneccessary ManuscriptreceivedAugust18,2011;acceptedforpublicationNovember9,2011 This is an open-access article distributed under the terms of the Creative sequences and are optimized for enhancer detection due to the CommonsAttributionUnportedLicense(http://creativecommons.org/licenses/ positionofthecloningsite,inclusionofinsulators,anduseofmul- by/3.0/),whichpermitsunrestricteduse,distribution,andreproductioninany tiple reporters. medium,providedtheoriginalworkisproperlycited. To achieve this,weadaptedelementsfromtheexistingHZ50PL- 1Correspondingauthor:DepartmentofPhysiology,Development,and lacZenhancer–detectingvector(HiromiandGehring1987)andahigh Neuroscience,UniversityofCambridge,DowningStreet,CambridgeCB23DY, UK. E-mail:[email protected] copy p-element transformation plasmid [p-WhiteRabbit; Dunin- Volume2 | January 2012 | 79 Borkowski and Brown (1995)]. We combined the hsp70 minimal Vectorsaccurately reportNotchresponsive promoter from HZ50PL-lacZ with eGFP, mCherry, lacZ, or venus enhanceractivity [PEST]-YFP coding sequences. Incorporating these reporters into To test the functionality of these vectors, we inserted a previously a plasmid containing the p-WhiteRabbit vector backbone, mini- characterized Notch responsive element (NRE) (Furriols and Bray white, and kanamycin resistance genes (kan) in combination with 2001). Costaining to detect expression from NRE-GreenRabbit and anattBsequenceenablesuseoftheFC31system.Alox-psitewas the previous NRE-lacZ (Figure 2, B-B”) revealed identical patterns included to allow removal of kan and platform sequences after in wing discs. Furthermore, NRE-GreenRabbitgavethe expected ex- genomicintegration. pression patterns elsewhere. In trachea, GFP was detected only in Tominimizeinfluencefrompositioneffects,themini-whitegene nestsofcellsatthetrachealbranchpoints,asreportedfortheparent and vector backbone are arranged to flank the reporter gene after NRE reporter (Furriols and Bray 2001), and in larval brains, it was integration (Figure 1). We also inserted insulator (gypsy) elements, present in imaginal neuroblasts, a known site of Notch activity which have been shown to be effective in reducing the influence of (Almeida and Bray 2005) (Figure 2, I and J). Notch responsiveness neighboring sequences, flanking mini-white and the reporter gene of NRE-GreenRabbit was confirmed by expressing Notch-RNAi in (Barolo et al. 2000; Barolo et al. 2004) (Figure 1, purple circles). posterior compartments of wing discs. Under these conditions, ex- Resulting vectors are named after the originating plasmid pression waslost, indicatingthatit is dependenton Notch signaling (pWhiteRabbit), substituting the color prefix according to the type (Figure2F).NREfunctionwasalsoaccuratelyreportedwithmCherry, ofreporter (pGreenRabbit, etc.). Thesevectors arecompatible with lacZ, and Venus[PEST]-YFP variants (Figure 2, C-E). As expected, a wide range of experiments, including live imaging. For example, independent insertions of NRE-RedRabbit at a single platform site destabilized Venus[PEST]-YFP could be used when perdurance of gave reproducible expression levels compared with independent the reporter would be an issue or when fine-scale temporal differ- NRE-lacZ p-element insertions (Figure 2K). The new vectors, there- encesinexpressionareinvestigated(Aulehlaetal.2008;Nagaietal. fore, accurately and reproducibly report known expression patterns 2002).Furthermore,thedifferentreportersenableseveralregulatory fromenhancerelements.Thelinesgeneratedwillalsoprovideuseful elementstobeanalyzed simultaneously. toolsforanalysisofNotchpathwayactivityinvivo. Reportersshowno basalexpression Transgenesareresistant topositioneffects One important criterion for reporter constructs is that basal Totestsusceptibilitytosurroundingsequences,weanalyzedexpression expression levels should be low. We tested whether pGreenRabbit from pGreenRabbit at a location prone to position effects from a gave any expression in the absence of an enhancer by generating neighboring gene (51D) (http://flyc31.frontiers-in-genetics.org/). No ex- insertionsinseveralattPplatformlines(2A,22A,51D,68E,81C,and pression was detected in wing imaginal discs (Figure 3A) or in several 96E).InnocasewasGFPexpressiondetectedinthewingdisc(Figure other tissues (Figure 2, G and H), indicating that the flanking vector 2A and data not shown). Similarly, no basal expression could be sequencesareeffectivebuffers.Whenthesevectorswereremovedbyin- detected in larval brains or trachea, confirming their efficacy as en- ducingrecombinationbetweenlox-psites,patternedreporterexpression hancer-detectionvectors(Figure2,GandH). waspresentbutgreatlyattenuatedinthepresenceofinsulators(Figure3, Figure1 Reportervectorscom- patiblewithFC31transgenesis techniques. Diagram of vector backbone (top) into which four different reporters have been inserted as indicated. All vec- tors carry kanamycin resistance andusemini-whiteasatransfor- mationmarker.Allreportersare downstreamofaminimalhsp70 promoter and are flanked by UTRs from the hsp70 gene. The positions of gypsy (SuHw) insulator sequences (purple), lox-p, attB (yellow), and multi- ple cloning site (MCS) unique restrictionsitesareindicated. 80 | B.Housden,K.Millen,andS.J.Bray Figure2 VectorsaccuratelyreportexpressionpatternfromaNotchresponsiveelement.(A)BasalexpressionfrompGreenRabbit(GR)integrated atplatform51D.(B–E)ExpressionfromindicatedreportervectorsdrivenbytheNotchresponsiveelement(NRE)inthewingpouchofthirdinstar larvae.NRE-lacZ(B,magenta;B99,white)isapreviouslyreportedNotchreporter(FurriolsandBray2001).ThesameNREwasusedtogenerate NRE-GreenRabbit(NRE-GRins;B,green;B9,white);NRE-RedRabbit(NRE-RRins;C);NRE-BlueRabbit(NRE-BRins;D);andNRE-VenusRabbit(NRE- VRins;E).NRE-VRinswasimagedwith10·excitation.(F)Notch-RNAiexpressionintheposteriorcompartment(greenbraces;drivenusingen- Gal4)eliminatesexpressionfromNRE-GRins.(G,H)BasalexpressionfrompGRintegratedatplatform51Dinthelarvalbrain(G)andtrachea(H).(I, J)ExpressionfromNRE-GRinsinthelarvalbrain(I)andtrachea(J).Suffix“ins”indicatesthattheconstructscontainedinsulators.(K)Comparisonof expressionlevelsfromindependenttransgeniclines(averagepixelintensityinthewingpouchmeasuredusingImageJ).NRE-RRinsertionsatthe sameplatform(86Fb)producesimilarexpressionlevels.NRE-lacZinsertionsgeneratedusingp-elementtransgenesisareexpressedatvarying levels. At least five discs were quantified per genotype. Error bars show standard error of the mean. Primary antibodies were rabbit a-GFP (MolecularProbes,1/500)(A,B,andE–J);rabbita-dsRed(ClonTech,1/50)(C);andmousea-bGalactosidase(DevelopmentalStudiesHybridoma Bank,1/20)(BandD). B-C).Therefore,boththebufferingsequencesandinsulatorsareeffective Insummary,wehaveconstructedaseriesoffourreportervectors inpreventingpositioneffectsandmakethevectorsresistanttoinfluences specifically designed for use with FC31-mediated transgenesis that fromsurroundingDNA.Furthermore,theinsulatorsequenceshaveno enable analysis and direct comparisons of different enhancers. Insu- adverseeffectsonvectorfunction,(Figure3,DandE). lator elements and buffering sequences have been incorporated to Volume2 January2012 | FC31-CompatibleReporterVectors | 81 Aulehla,A.,W.Wiegraebe,V.Baubet,M.B.Wahl,C.Dengetal.,2008 A beta-cateningradientlinkstheclockandwavefrontsystemsinmouse embryosegmentation.Nat.CellBiol.10:186–193. 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