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Drosophila pVALIUM10 TRiP RNAi lines cause undesired silencing of Gateway-based transgenes

Dimitrije Stanković, Gábor Csordás, Mirka Uhlirova  Correspondence email
Published 29 November 2022. DOI: 10.26508/lsa.202201801

Abstract

Post-transcriptional gene silencing using double-stranded RNA has revolutionized the field of functional genetics, allowing fast and easy disruption of gene function in various organisms. In Drosophila, many transgenic RNAi lines have been generated in large-scale efforts, including the Drosophila Transgenic RNAi Project (TRiP), to facilitate in vivo knockdown of virtually any Drosophila gene with spatial and temporal resolution. The available transgenic RNAi lines represent a fundamental resource for the fly community, providing an unprecedented opportunity to address a vast range of biological questions relevant to basic and biomedical research fields. However, caution should be applied regarding the efficiency and specificity of the RNAi approach. Here, we demonstrate that pVALIUM10-based RNAi lines, representing ∼13% of the total TRiP collection (1,808 of 13,410 pVALIUM TRiP–based RNAi lines), cause unintended off-target silencing of transgenes expressed from Gateway destination vectors. The silencing is mediated by targeting attB1 and attB2 sequences generated via site-specific recombination and included in the transcribed mRNA. Deleting these attB sites from the Gateway expression vector prevents silencing and restores expected transgene expression.

Introduction

dsRNA-mediated post-transcriptional gene silencing, also known as RNAi, represents an ancient antiviral defense mechanism that has been harnessed as a powerful tool for reverse functional genetics in various cultured cells, and plant and animal model systems (Kennerdell & Carthew, 1998; Lohmann et al, 1999; Wargelius et al, 1999; Wianny & Zernicka-Goetz, 2000; Zamore et al, 2000). The dsRNA silencing relies on a highly conserved RNase III enzyme called Dicer that recognizes and processes dsRNA into small 21- to 23-bp segments (siRNA). Upon loading into a multiprotein RNA-induced silencing complex, the guide strand facilitates pairing with complementary on-target RNAs, which are subsequently degraded by the action of Argonaut proteins (Tomari & Zamore, 2005). In Drosophila, spatiotemporally controlled RNAi knockdown can be achieved by expressing dsRNA using transgenic binary expression systems, such as Gal4/UAS (Brand & Perrimon, 1993). The initial transgenic RNAi lines were generated using plasmids with ligated inverted repeats transcribed from one (Kennerdell & Carthew, 1998) or two (Giordano et al, 2002) opposite promoters. However, these vectors were unstable and not well tolerated by the bacterial strains commonly used for cloning (Hagan & Warren, 1983; Piccin et al, 2001), a problem later solved by the introduction of an intron spacer between the repeats (Lee & Carthew, 2003; Bao & Cagan, 2006). This step-by-step progress led to the development of the pVALIUM (vermilion-attB-loxP-intron-UAS-MCS), a universal vector system for transgenic RNAi library generation. The pVALIUM RNAi vectors contain an eye-color selection marker (vermillion), an attB site enabling phiC31-mediated site-directed integration into predefined genomic locations, white or ftz introns promoting the processing of dsRNA, and a cassette of two UAS pentamers, one of which is flanked by loxP sites to allow tuning of the dsRNA expression levels, and multiple cloning sites (MCSs) (Ni et al, 2008).

The highly efficient pVALIUM10-based transgenic RNAi stocks produced within the Drosophila Transgenic RNAi Project (TRiP; https://fgr.hms.harvard.edu/fly-in-vivo-rnai) at Harvard Medical School (HMS) https://fgr.hms.harvard.edu represent an invaluable resource for the Drosophila community (Perkins et al, 2015). At the moment of writing, 1,808 transgenic TRiP RNAi stocks based on the pVALIUM10 are available at the Bloomington Drosophila Stock Center (BDSC; https://bdsc.indiana.edu/index.html) (Perrimon et al, 2010). The pVALIUM10 vector carries gypsy insulators that markedly enhance knockdown efficiency, along with two inverted “attR1-selection-attR2” cassettes that facilitate cloning of dsRNA fragments via site-specific Gateway in vitro recombineering (Ni et al, 2009; Reece-Hoyes & Walhout, 2018). A desired single fragment, 400–600 bp in length and flanked by attL1 and attL2 recombination sites, can be easily moved from an entry vector into a pVALIUM10 destination vector via recombination between attL and attR sites catalyzed by LR Clonase, producing a vector for the UAS-driven expression of dsRNA (Ni et al, 2009).

The Gateway cloning technology is also routinely used to generate transgenic constructs for the expression of epitope-tagged or untagged proteins, taking advantage of the Drosophila Gateway plasmid collection at the Drosophila Genomics Resource Center (DGRC; https://dgrc.bio.indiana.edu/). Importantly, as with pVALIUM10 dsRNA plasmids, production of Gateway expression vectors relies on the recombination between attL and attR sites resulting in the formation of attB1 and attB2 sites.

Here, we demonstrate that the pVALIUM10-derived RNAi lines cause undesirable knockdown of transgenic reporters and overexpression lines generated with the help of the Gateway cloning technology. They do so by targeting the attB sites that are part of the transcribed mRNA. Deletion of the attB1 and attB2 sequences from the Gateway expression destination vector abrogates this effect and restores expected transgene expression levels.

Results

Unexpected, off-target silencing of the RNase H1::GFP reporter by multiple pVALIUM10 RNAi lines

In vivo RNAi-based genetic screens have proved very successful in identifying novel genes involved in developmental and pathologic processes in a variety of Drosophila somatic tissues when expressed using tissue-specific Gal4 driver lines (Lesch et al, 2010; Neely et al, 2010; Saj et al, 2010; Port et al, 2011; Zeng et al, 2015; Pletcher et al, 2019; Rotelli et al, 2019; Zhou et al, 2019; Graca et al, 2021; Rylee et al, 2022). Hence, we embarked on a candidate genetic screen aimed at identifying factors controlling genome stability. During the pre-screening of potential candidates, we observed that the expression of pVALIUM10-based BuGZRNAi[TRiP.JF02830] RNAi line in the pouch region of the developing third instar wing discs, using the nubbin-Gal4, UAS-mRFP (nub > mRFP) driver line, efficiently suppressed the multi-epitope–tagged BuGZ transgene (BuGZFlyFos[v318366]) (Sarov et al, 2006) (Fig 1A, B, and D). A similar reduction was observed using an independent BuGZRNAi[KK104498] line from the Vienna Drosophila Resource Center (VDRC) KK RNAi library (Fig 1C and D). Encouraged by these results, both BuGZ RNAi lines were included in the candidate genetic screen that was based on the expression of selected dsRNAs with the nub > mRFP driver. As readout for genome stability, we used the ubiquitously driven RNase H1::GFP that was generated by recombining the RNase H1 coding sequence into the pUWG vector from the Drosophila Gateway plasmid collection. This resulted in the expression of a C-terminally GFP-tagged RNase H1 under the control of the polyubiquitin promoter (Fig 2A and B). The RNase H1 enzyme recognizes and resolves R-loops, DNA:RNA hybrids, that emerge during transcription and represent a threat to genome stability when unresolved (Santos-Pereira & Aguilera, 2015; Crossley et al, 2019). Unexpectedly, we observed a reduction in RNase H1::GFP signal when expressing BuGZRNAi[TRiP.JF02830] but not BuGZRNAi[KK104498] line (Fig 2C, D, and H). Strikingly, similar down-regulation of RNase H1::GFP was caused by pVALIUM10-based mycRNAi[TRiP.JF01761] but not mycRNAi[TRiP.HMS01538] or mycRNAi[GD2948] derived from pVALIUM20 and pMF3 vectors, respectively (Figs 1D and 2E–H). All three myc RNAi lines have been shown effective by others (Aughey et al, 2016; Kim-Yip & Nystul, 2018; Rust et al, 2018; Ledru et al, 2022). These results indicated that the tested pVALIUM10 TRiP RNAi lines but not pVALIUM20, KK, or GD lines may cause undesirable silencing of the RNase H1::GFP transgene. We further speculated that dsRNA expressed from pVALIUM10 contains segments unrelated to the target gene-specific sequences that trigger this unexpected off-target effect.

Figure 1.
Figure 1. pVALIUM10 and KK RNAi lines cause efficient silencing.

(A, B, C) Expression of pVALIUM10 BuGZRNAi[TRIP.JF02830] (B, B’) and KK-based BuGZRNAi[KK104498] transgenic RNAi lines (C, C’) using the nubbin-Gal4, UAS-myr-mRFP driver (nub > mRFP, light blue) causes a marked reduction in a BuGZFlyFos[v318366] transgenic protein in the pouch region of wing discs (WDs) relative to the hinge and notum, and control WD (A, A’). Micrographs show projections of multiple confocal sections of WDs dissected from third instar larvae 7 d AEL. The multi-epitope–tagged BuGZFlyFos [v318366] protein was visualized by immunostaining with an anti-GFP antibody (white). Nuclei were counterstained with DAPI (magenta). Scale bars: 100 µm. (D) Schematic representation of various vectors used for cloning and overexpression of dsRNA. In the absence of the target-specific antibody, the RNAi efficacy can be assessed with the help of FlyFos transgenes expressing multi-epitope–tagged proteins under the control of the endogenous regulatory sequences.

Figure 2.
Figure 2. pVALIUM10-based lines cause off-target silencing of the RNase H1::GFP transgenic reporter.

(A) Schematic representation of the transgenic pUWG-RNase H1 reporter construct expressing the C-terminally GFP-tagged RNase H1::GFP protein from the polyubiquitin (ubi) promoter. The RNase H1 coding sequence is flanked by attB1 and attB2 sites generated via Gateway-mediated recombination catalyzed by the LR Clonase. (B, C, D, E, F, G) Immunostaining with a GFP-specific antibody revealed a marked reduction of the RNase H1::GFP levels in the nubbin domain (mRFP, light blue), where pVALIUM10-based BuGZRNAi[TRIP.JF02830] (C) and mycRNAi[TRiP.JF01761] (E) RNAi lines were expressed using the nubbin-Gal4, UAS-myr-mRFP driver (nub > mRFP). No such down-regulation of the RNase H1::GFP signal was observed in control WD (B) and after expression of KK-based BuGZRNAi[KK104498] (D), pVALIUM20-based mycRNAi[TRiP.HMS01538] (F), or GD-based mycRNAi[GD2948] (G). Micrographs show projections of multiple confocal sections of WDs dissected from third instar larvae 7 d AEL. Nuclei were counterstained with DAPI (magenta). Scale bars: 100 µm. (H) Quantification of the RNase H1::GFP signal depicted as a relative intensity ratio between the pouch and the notum region. Statistical significance was determined by one-way ANOVA with Tukey’s multiple comparison test; n ≥ 3; **P < 0.01, ****P < 0.0001, and n.s., non-significant. (I) Generation of pVALIUM10 RNAi lines relied on a LR Clonase–mediated recombination of dsRNA fragment from an entry vector to the pVALIUM10 destination vector (Ni et al, 2009). The dsRNA hairpin produced from the pVALIUM10 dsRNA expression vector is the source of siRNA species targeting not only the transcript of interest (target ORF) but also attB1 and attB2 sites present in any of the Gateway expression vectors generated via the same recombination mechanisms.

Source data are available for this figure.

Source Data for Figure 2[LSA-2022-01801_SdataF2.xlsx]

pVALIUM10 RNAi and Gateway expression plasmids share attB recombination sites

To identify the potential target for dsRNA-mediated knockdown of the RNase H1::GFP transgene by pVALIUM10 TRiP RNAi, we compared the plasmid sequences. We found that attB1 and attB2 sites are shared between the Gateway-based expression vectors, including pUWG, and pVALIUM10 TRiP RNAi plasmids. attB1 and attB2 sites are 25 bp in length and generated by LR Clonase–mediated recombination between attL and attR sequences. Given the repetition of attB1 and attB2 sites, flanking the passenger and guide target sequence fragments in pVALIUM10 TRiP RNAis, these sequences are transcribed and could contribute to the dsRNA stem–loop substrate for Dicer. Based on these results, we hypothesized that dsRNAs generated from attB1 and attB2 could target, and thus silence, Gateway-based transgenes via attB sites (Fig 2I).

pVALIUM10 RNAi lines silence Gateway transgenes via attB sites

To test our hypothesis, we cloned the mCherry coding sequence into the pUWG Gateway expression vector (pUWG-mCherry) allowing the ubiquitous expression of mCherry transcript flanked by the attB1 and attB2 sites. The pUWG-mCherry vector then served as a template for overlap PCR to generate the pUWGΔattB-mCherry construct that lacks attB sites (Fig 3A). Both plasmids were used to establish transgenic fly lines through a standard Drosophila germline transformation method (Rubin & Spradling, 1982). The susceptibility or resistance of ubi-mCherry (pUWG-mCherry) and ubiΔattB-mCherry (pUWGΔattB-mCherry) transcripts to RNAi-mediated silencing was then tested by driving various RNAi lines under the control of the nub-Gal4 driver. Immunostaining of the third instar wing imaginal discs using an anti-RFP antibody revealed an identical pattern of ubi-mCherry and ubiΔattB-mCherry transgenes in the control (nub>) background (Fig 3B and C). In contrast, levels of ubi-mCherry but not ubiΔattB-mCherry transgenic protein were markedly reduced in the wing pouch region relative to the rest of the tissue after overexpression of BuGZ and myc pVALIUM10 TRiP RNAi lines (Fig 3D, E, H–J, and M), whereas no significant changes were observed when BuGZ and myc were knocked down using KK and pVALIUM20 RNAi lines, respectively (Fig 3F–H and K–M). Importantly, the attB site–dependent silencing of ubi-mCherry was recapitulated using an additional set of pVALIUM10 TRiP RNAi lines targeting Atf3, Lip4, yki, DH44, ftz-f1, mago, brat, and Actβ genes (Fig S1).

Figure 3.
Figure 3. pVALIUM10 RNAi lines silence Gateway transgenes via attB1 and attB2 sites.

(A) Schematic of the transgenic pUWG-mCherry and mutant pUWGΔattB-mCherry reporter constructs. The mCherry is expressed from the polyubiquitin (ubi) promoter. (B, C) ubi-mCherry and mutant ubiΔattB-mCherry reporters showed a similar expression pattern in the wing imaginal discs. (D, E, F, G, H, I, J, K, L, M) ubi-mCherry was efficiently down-regulated by pVALIUM10 BuGZRNAi[TRIP.JF02830] and mycRNAi[TRiP.JF01761] expressed under the control of the nubbin-Gal4 driver (nub>) relative to the rest of the WD (D, H, I, M). (E, H, J, M) In contrast, the absence of attB1 and attB2 sequences rendered the ubiΔattB-mCherry reporter resistant to pVALIUM10 RNAi–mediated silencing (E, H, J, M). (F, G, H, K, L, M) Neither KK-based (BuGZRNAi[KK104498]) nor pVALIUM20-based (mycRNAi[TRiP.HMS01538]) RNAi lines affected mCherry levels expressed from the unmodified or mutant reporter constructs (F, G, H, K, L, M). Micrographs show projections of multiple confocal sections of WDs dissected from third instar larvae 7 d AEL that were immunostained with an anti-mRFP antibody (white). Nuclei were counterstained with DAPI (magenta). Scale bars: 100 µm. (H, M) Quantification of the mCherry signal depicted as a relative intensity ratio between the pouch and the notum region (H, M). Superscript text in each group denotes the type of RNAi used. Statistical significance was determined by one-way ANOVA with Tukey’s multiple comparison test; n ≥ 3; **P < 0.01, ****P < 0.0001, and n.s., non-significant. (N, O, P, Q) Expression of pVALIUM10 BuGZRNAi[TRIP.JF02830] (O) in the wing pouch using the nubbin-Gal4, UAS-mRFP driver (nub > mRFP) reduces SmD3::3xHA levels compared with control (N) and KK-based BuGZRNAi[KK104498] (P). Note foci of SmD3::3xHA protein in control (N”) and BuGZRNAi[KK104498] (P”) cells that are not present in BuGZRNAi[TRIP.JF02830]-expressing cells (O”). Micrographs show projections of multiple or single (N”, O”, P”) confocal sections of WDs dissected from third instar larvae 7 d AEL that were immunostained with an anti-HA antibody (white, N’, O’, P’; red, N”, O”, P”). Nuclei were counterstained with DAPI (magenta). Scale bars: 100 or 5 μm (N”, O”, P”). (Q) Quantification of the SmD3::3xHA signal intensity (Q, left) and SmD3::3xHA-positive punctae (Q, right) in the pouch region. Statistical significance was determined by one-way ANOVA with Tukey’s multiple comparison test and Kruskal–Wallis test, respectively; n ≥ 6; **P < 0.01, ***P < 0.001, and n.s., non-significant.

Source data are available for this figure.

Figure S1.
Figure S1. pVALIUM10 RNAi lines silence Gateway transgenes via attB1 and attB2 sites.

(A, B, C, D, E, F, G, H, I, J, K, L, M, N, O, P) WT ubi-mCherry but not the ubiΔattB-mCherry reporter lacking attB1 and attB2 sequences was efficiently down-regulated in the pouch region by pVALIUM10 RNAi lines targeting Atf3 (A, B), yki, (C, D), Actβ (E, F), ftz-f1 (G, H), DH44 (I, J), Lip4 (K, L), mago (M, N), and brat (O, P) transcripts expressed under the control of the nubbin-Gal4 driver (nub>) relative to the rest of the WD. Micrographs show projections of multiple confocal sections of WDs dissected from third instar larvae 7 d AEL that were immunostained with an anti-mRFP antibody (white). Nuclei were counterstained with DAPI (magenta). Crosses were maintained at 29°C. Scale bars: 100 µm.

Finally, we tested whether pVALIUM10 TRiP RNAi lines may also interfere with UAS-inducible attB-containing transcripts, such as transgenic fly ORFs expressed from the Gateway destination vector pGW-HA.attB (Bischof et al, 2014). To this end, we assessed levels of the SmD3::3xHA protein in the presence of the pVALIUM10 or KK BuGZ-RNAi line. In contrast to an enrichment of SmD3::3xHA protein and positive punctae in the wing pouch cells of control (nub>) and BuGZRNAi[KK104498] expressing wing discs, the overall levels and the number of positive punctae were noticeably reduced in nub > BuGZRNAi[TRiP.JF02830] cells (Fig 3N–Q). These results suggest that the dsRNA hairpin produced from pVALIUM10 RNAi vectors generates attB1- and attB2-siRNAs, which guide destruction of transcripts containing such target sites. This off-target silencing via attB sites is specific to RNAi lines based on pVALIUM10. The absence of attB1 and attB2 sites renders the Gateway-derived transcript resistant to unintended pVALIUM10 TRiP RNAi silencing.

Discussion

The use of transgenic RNAi to achieve developmental stage- and tissue-specific knockdown of candidate genes and to perform genome-wide screening in Drosophila has become commonplace in the past two decades (Dietzl et al, 2007; Port et al, 2011; Blake et al, 2017; Hu et al, 2017). Both our knowledge of the RNAi mechanism and the tools to generate new types of RNAi constructs efficiently have considerably evolved in recent years. As a result, several independent transgenic RNAi stock collections were established, including Vienna Drosophila Stock Center (VDRC, 23,411 RNAi lines; https://stockcenter.vdrc.at/control/main), Bloomington Drosophila Stock Center (BDSC, 13,698 RNAi lines; https://bdsc.indiana.edu/), and the National Institute of Genetics (NIG, 12,365 RNAi lines; https://shigen.nig.ac.jp/fly/nigfly/) at the time of writing. Yet, in spite of being a broadly used technique, transgenic manipulation of gene expression can still have unforeseen consequences. A large portion of the RNAi lines from the VDRC KK collection were found to produce phenotypes because of a secondary insertion and consequent ectopic expression of the tiptop gene (Green et al, 2014; Vissers et al, 2016). More recently, van der Graaf and colleagues reported that transgenes inserted in the commonly used attP40 landing site on the second chromosome can decrease the expression of Msp300, a member of the LINC complex, and hence lead to nuclear size, shape, and positioning phenotypes (van der Graaf et al, 2022 Preprint).

Here, we demonstrate that the pVALIUM10-based RNAi lines cause off-target silencing of ORFs expressed from Gateway expression vectors or potentially any transcripts containing attB1 and attB2 sites. We show that the removal of these sites abrogates the undesirable knockdown. Given the popularity of the Gateway expression vectors to generate transgenic protein reporters and tagged overexpression constructs, our results suggest that the simultaneous use of pVALIUM10 TRiP RNAi may lead to experimental artifacts unrelated to the investigated biological process.

Of note, in the original publication of pVALIUM10 vectors, the authors tested for potential off-target effects by comparing the hairpin sequence against the Drosophila genome (Ni et al, 2009), which does not contain endogenous 21-nt stretches equivalent to the attB1 and attB2 sequences. However, as the transgenic toolkit in Drosophila is ever expanding, each additional transgene has the possibility to produce a synthetic effect with the existing RNAi lines. Hence, we suggest that the researchers validate the type of the TRiP RNAi line or the expression vector sequence before commencing their experiments. As an example, we do not recommend combining RNAi based on pVALIUM10 with the 3xHA-tagged overexpression lines from FlyORF (https://flyorf.ch) (Bischof et al, 2014) or the fly-FUCCI (fluorescent ubiquitination-based cell cycle indicator) lines, which allow real-time visualization of the cell cycle dynamics by the expression of two fluorescently-tagged degrons (Zielke et al, 2014). In both cases, the transgenes were generated via Gateway reaction and contain attB sites flanking the inserted ORF (Bischof et al, 2014; Zielke et al, 2014), which can lead to off-target silencing of the transcript. Furthermore, this finding reinforces the idea that RNAi experiments should adhere to the standards established in the past decades, including investigating possible off-target effects to eliminate knockdown of the unintended gene, using multiple independent RNAi lines to recapitulate phenotypes, and confirming the knockdown of the targeted gene products (Echeverri et al, 2006; Green et al, 2014; Kaya-Çopur & Schnorrer, 2016).

Materials and Methods

Fly stocks and husbandry

The following Drosophila strains were used: w1118 (BDSC; RRID: BDSC_3605), nubbin-Gal4, UAS-myr-mRFP (nub > mRFP), BuGZFlyFos[v318366] (VDRC), BuGZRNAi[TRiP.JF02830] (BDSC; RRID:BDSC_27996), BuGZRNAi[KK104498] (VDRC), Lip4RNAi[TRiP.HMO5136] (BDSC; RRID:BDSC_28925), mycRNAi[TRiP.JF01761] (BDSC; RRID:BDSC_25783), mycRNAi[TRiP.HMS01538] (BDSC; RRID:BDSC_36123), mycRNAi[GD2948] (VDRC), ActβRNAi[TRiP.JF03276] (BDSC; RRID:BDSC_29597), ftz-f1RNAi[TRiP.JF02738] (BDSC; RRID:BDSC_27659), ykiRNAi[TRiP.JF03119] (BDSC; RRID:BDSC_31965), Atf3RNAi[TRiP.JF02303] (BDSC; RRID:BDSC_26741), DH44RNAi[TRiP.JF01822] (BDSC; RRID:BDSC_25804), bratRNAi[TRiP.HM05078] (BDSC; RRID:BDSC_28590), magoRNAi[TRiP.HM05142] (BDSC; RRID:BDSC_28931), SmD3::3xHA[FlyORF F003987] (FlyORF), and ubi-RNase H1::GFP, ubi-mCherry, and ubiΔattB-mCherry (this study). All Drosophila stocks are listed in Table S1. All crosses were set up and maintained at 25°C, unless specified otherwise, on a diet consisting of 0.8% agar, 8% cornmeal, 1% soymeal, 1.8% dry yeast, 8% malt extract, and 2.2% sugar–beet syrup, which was supplemented with 0.625% propionic acid and 0.15% Nipagin. w1118 line was used as a control.

Generation of plasmids and transgenic lines

The ORF of rnh1 (FBgn0023171) was amplified from Drosophila melanogaster cDNA (w1118) using primers harboring NotI and SalI restriction sites. The stop codon was excluded to allow C-terminal tagging of the protein. The ORF was cloned into the Gateway pENTR 4 Dual Selection vector (Cat# A10465; Thermo Fisher Scientific). The ORF was then recombined into the pUWG vector (Cat# 1284; DGRC) using the LR Clonase II enzyme mix according to manufacturer’s instructions (Cat# 11791020; Thermo Fisher Scientific). The coding sequence of mCherry (GenBank: AY678264.1) was amplified with specific primers, cloned into the pENTR 4 Dual Selection vector (Cat# A10465; Invitrogen) including a stop codon, and subsequently recombined into the pUWG vector (pUWG-mCherry). Overlap PCR strategy was employed to generate the pUWGΔattB-mCherry construct lacking attB sites resulting from the LR recombination. Three separate PCRs were performed to produce fragments for assembly using the original pUWG-mCherry plasmid as a template. The forward primer of the first primer pair contained a XhoI restriction site, whereas the reverse primer contained a XbaI restriction site. Partial complementarity of the reverse and forward primers used to synthesize the downstream fragment enabled the exclusion of attB sites in the final product. The final PCR product was ligated into the pUWG-mCherry plasmid digested with XbaI and XhoI. Transgenic fly lines with random insertions of the constructs were generated by standard P-element–mediated transformation using the w1118 Drosophila strain. All primers and plasmids are listed in Table S2.

Tissue dissection and immunostaining

Wing imaginal disks dissected from third instar Drosophila larvae (7 d after egg laying) were fixed for 25 min with 4% paraformaldehyde in PBS containing 0.1% Triton X (PBS-T) at room temperature. Fixed tissues were washed three times with PBS-T. Primary antibodies were diluted in blocking buffer (PBS-T with 0.3% BSA), and tissues were stained overnight at 4°C. The following primary antibodies were used: rabbit anti-mRFP (1:500, Cat# PM005, RRID:AB_591279; MBL International), goat anti-GFP (1:500, Cat# ab6673, RRID:AB_305643; Abcam), and rabbit-anti HA (1:1,000, Cat# ab9110, RRID:AB_307019; Abcam). After washing, the samples were incubated with the corresponding Alexa Fluor 488 (1:2,000, Cat# A-11034, RRID:AB_2576217; Thermo Fisher Scientific)–, Cy2 (1:2,000, Cat# 705-225-147, RRID:AB_2307341; Jackson ImmunoResearch Labs)-, or Cy3 (1:2,000, Cat# 711-165-152, RRID:AB_2307443; Jackson ImmunoResearch Labs)-conjugated secondary antibodies overnight at 4°C, and washed and counterstained with DAPI (1:1,000 dilution of 5 mg/ml stock, Cat# 6335.1; Carl Roth GmbH) to visualize nuclei. Tissues were mounted on glass slides in DABCO–Mowiol 4-88 (Cat# D2522 and Cat# 81381; Sigma-Aldrich).

Image acquisition and processing

Confocal images and stacks were acquired with an Olympus FV1000 confocal microscope equipped with 20× UPlan S-Apo (NA 0.85), 40× UPlan FL (NA 1.30), and 60× UPlanApo (NA 1.35) objectives. Maximum Z-projections were generated from consecutive sections taken at 1.4-µm steps using the FluoView 1000 software (Olympus) (RRID: SCR_014215) and Fiji (https://fiji.sc/) (RRID:SCR_002285). Final image processing, including panel assembly, and brightness and contrast adjustments were performed in Adobe Photoshop CC (Adobe Systems, Inc.) (RRID:SCR_014199). The schemes were generated in Adobe Illustrator CC (Adobe Systems, Inc.) (RRID:SCR_010279) and BioRender.com (RRID:SCR_018361; BioRender).

Quantification of mCherry, RNase H1::GFP, and SmD3::3xHA signal

Fluorescent signal intensity was quantified with Fiji (https://fiji.sc/) (RRID:SCR_002285). For mCherry and RNase H1::GFP, a square selection was created in the middle of the pouch region, and the mean intensity was measured; then, the same selection was moved to the middle of the notum, and the measurement was repeated. The two values were divided to produce a pouch/notum intensity ratio for each wing disc. For SmD3::3xHA, the mean intensities of SmD3::3xHA and mRFP signals in the pouch region were measured and divided to produce a normalized value for each wing disk. Zoom images of the nubbin domain of independent WDs were used to count the number of SmD3::3xHA-positive punctae per 1,000-µm2 area. Statistical significance was determined by one-way ANOVA with Tukey’s multiple comparison test (signal intensity) or Kruskal–Wallis test (punctae) in GraphPad Prism (RRID:SCR_002798).

Acknowledgements

We thank Norbert Perrimon for discussions and comments on the article. We thank the Bloomington Drosophila Stock Center (BDSC, Bloomington, IN, USA), the Vienna Drosophila Resource Center (VDRC, Vienna, Austria), the Drosophila Genomic Resource Center (DGRC, supported by NIH grant 2P40OD010949, Bloomington, IN, USA), and the Zurich ORFeome Project (FlyORF, Zurich, Switzerland) for fly stocks and plasmids. We are grateful to Tina Bresser for generation of transgenic lines and Nils Teuscher for fly stock maintenance and technical assistance. This work was funded by the Deutsche Forschungsgemeinschaft (DFG, German Research Foundation) under Germany’s Excellence Strategy – CECAD (EXC 2030 – 390661388).

Author Contributions

  • D Stanković: resources, formal analysis, validation, investigation, visualization, methodology, and writing—original draft, review, and editing.

  • G Csordás: conceptualization, formal analysis, validation, methodology, and writing—original draft, review, and editing.

  • M Uhlirova: conceptualization, resources, data curation, formal analysis, supervision, funding acquisition, validation, investigation, visualization, methodology, and writing—original draft, review, and editing.

Conflict of Interest Statement

The authors declare that they have no conflict of interest.

  • Received November 3, 2022.
  • Revision received November 14, 2022.
  • Accepted November 16, 2022.
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This article is available under a Creative Commons License (Attribution 4.0 International, as described at https://creativecommons.org/licenses/by/4.0/).

References

    1. Aughey GN,
    2. Grice SJ,
    3. Liu J-L
    (2016) The interplay between Myc and CTP synthase in Drosophila. PLoS Genet 12: e1005867. doi:10.1371/journal.pgen.1005867
    OpenUrlCrossRefPubMed
    1. Bao S,
    2. Cagan R
    (2006) Fast cloning inverted repeats for RNA interference. RNA 12: 20202024. doi:10.1261/rna.258406
    OpenUrlAbstract/FREE Full Text
    1. Bischof J,
    2. Sheils EM,
    3. Björklund M,
    4. Basler K
    (2014) Generation of a transgenic ORFeome library in Drosophila. Nat Protoc 9: 16071620. doi:10.1038/nprot.2014.105
    OpenUrlCrossRefPubMed
    1. Blake AJ,
    2. Finger DS,
    3. Hardy VL,
    4. Ables ET
    (2017) RNAi-based techniques for the analysis of gene function in Drosophila germline stem cells. Methods Mol Biol 1622: 161184. doi:10.1007/978-1-4939-7108-4_13
    OpenUrlCrossRef
    1. Brand AH,
    2. Perrimon N
    (1993) Targeted gene expression as a means of altering cell fates and generating dominant phenotypes. Development 118: 401415. doi:10.1242/dev.118.2.401
    OpenUrlAbstract
    1. Crossley MP,
    2. Bocek M,
    3. Cimprich KA
    (2019) R-loops as cellular regulators and genomic threats. Mol Cell 73: 398411. doi:10.1016/j.molcel.2019.01.024
    OpenUrlCrossRefPubMed
    1. Dietzl G,
    2. Chen D,
    3. Schnorrer F,
    4. Su KC,
    5. Barinova Y,
    6. Fellner M,
    7. Gasser B,
    8. Kinsey K,
    9. Oppel S,
    10. Scheiblauer S, et al.
    (2007) A genome-wide transgenic RNAi library for conditional gene inactivation in Drosophila. Nature 448: 151156. doi:10.1038/nature05954
    OpenUrlCrossRefPubMed
    1. Echeverri CJ,
    2. Beachy PA,
    3. Baum B,
    4. Boutros M,
    5. Buchholz F,
    6. Chanda SK,
    7. Downward J,
    8. Ellenberg J,
    9. Fraser AG,
    10. Hacohen N, et al.
    (2006) Minimizing the risk of reporting false positives in large-scale RNAi screens. Nat Methods 3: 777779. doi:10.1038/nmeth1006-777
    OpenUrlCrossRefPubMed
    1. Giordano E,
    2. Rendina R,
    3. Peluso I,
    4. Furia M
    (2002) RNAi triggered by symmetrically transcribed transgenes in Drosophila melanogaster. Genetics 160: 637648. doi:10.1093/genetics/160.2.637
    OpenUrlAbstract/FREE Full Text
    1. Graca FA,
    2. Sheffield N,
    3. Puppa M,
    4. Finkelstein D,
    5. Hunt LC,
    6. Demontis F
    (2021) A large-scale transgenic RNAi screen identifies transcription factors that modulate myofiber size in Drosophila. PLoS Genet 17: e1009926. doi:10.1371/journal.pgen.1009926
    OpenUrlCrossRef
    1. Green EW,
    2. Fedele G,
    3. Giorgini F,
    4. Kyriacou CP
    (2014) A Drosophila RNAi collection is subject to dominant phenotypic effects. Nat Methods 11: 222223. doi:10.1038/nmeth.2856
    OpenUrlCrossRefPubMed
    1. Hagan CE,
    2. Warren GJ
    (1983) Viability of palindromic DNA is restored by deletions occurring at low but variable frequency in plasmids of Escherichia coli. Gene 24: 317326. doi:10.1016/0378-1119(83)90092-6
    OpenUrlCrossRefPubMed
    1. Hu Y,
    2. Comjean A,
    3. Roesel C,
    4. Vinayagam A,
    5. Flockhart I,
    6. Zirin J,
    7. Perkins L,
    8. Perrimon N,
    9. Mohr SE
    (2017) FlyRNAi.org-the database of the Drosophila RNAi screening center and transgenic RNAi project: 2017 update. Nucleic Acids Res 45: D672D678. doi:10.1093/nar/gkw977
    OpenUrlCrossRefPubMed
    1. Kaya-Çopur A,
    2. Schnorrer F
    (2016) A guide to genome-wide in vivo RNAi applications in Drosophila. Methods Mol Biol 1478: 117143. doi:10.1007/978-1-4939-6371-3_6
    OpenUrlCrossRefPubMed
    1. Kennerdell JR,
    2. Carthew RW
    (1998) Use of dsRNA-mediated genetic interference to demonstrate that frizzled and frizzled 2 act in the wingless pathway. Cell 95: 10171026. doi:10.1016/s0092-8674(00)81725-0
    OpenUrlCrossRefPubMed
    1. Kim-Yip RP,
    2. Nystul TG
    (2018) Wingless promotes EGFR signaling in follicle stem cells to maintain self-renewal. Development 145: dev168716. doi:10.1242/dev.168716
    OpenUrlAbstract/FREE Full Text
    1. Ledru M,
    2. Clark CA,
    3. Brown J,
    4. Verghese S,
    5. Ferrara S,
    6. Goodspeed A,
    7. Su TT
    (2022) Differential gene expression analysis identified determinants of cell fate plasticity during radiation-induced regeneration in Drosophila. PLoS Genet 18: e1009989. doi:10.1371/journal.pgen.1009989
    OpenUrlCrossRef
    1. Lee YS,
    2. Carthew RW
    (2003) Making a better RNAi vector for Drosophila: Use of intron spacers. Methods 30: 322329. doi:10.1016/s1046-2023(03)00051-3
    OpenUrlCrossRefPubMed
    1. Lesch C,
    2. Jo J,
    3. Wu Y,
    4. Fish GS,
    5. Galko MJ
    (2010) A targeted UAS-RNAi screen in Drosophila larvae identifies wound closure genes regulating distinct cellular processes. Genetics 186: 943957. doi:10.1534/genetics.110.121822
    OpenUrlAbstract/FREE Full Text
    1. Lohmann JU,
    2. Endl I,
    3. Bosch TC
    (1999) Silencing of developmental genes in Hydra. Dev Biol 214: 211214. doi:10.1006/dbio.1999.9407
    OpenUrlCrossRefPubMed
    1. Neely GG,
    2. Kuba K,
    3. Cammarato A,
    4. Isobe K,
    5. Amann S,
    6. Zhang L,
    7. Murata M,
    8. Elmen L,
    9. Gupta V,
    10. Arora S, et al.
    (2010) A global in vivo Drosophila RNAi screen identifies NOT3 as a conserved regulator of heart function. Cell 141: 142153. doi:10.1016/j.cell.2010.02.023
    OpenUrlCrossRefPubMed
    1. Ni JQ,
    2. Markstein M,
    3. Binari R,
    4. Pfeiffer B,
    5. Liu LP,
    6. Villalta C,
    7. Booker M,
    8. Perkins L,
    9. Perrimon N
    (2008) Vector and parameters for targeted transgenic RNA interference in Drosophila melanogaster. Nat Methods 5: 4951. doi:10.1038/nmeth1146
    OpenUrlCrossRefPubMed
    1. Ni JQ,
    2. Liu LP,
    3. Binari R,
    4. Hardy R,
    5. Shim HS,
    6. Cavallaro A,
    7. Booker M,
    8. Pfeiffer BD,
    9. Markstein M,
    10. Wang H, et al.
    (2009) A Drosophila resource of transgenic RNAi lines for neurogenetics. Genetics 182: 10891100. doi:10.1534/genetics.109.103630
    OpenUrlAbstract/FREE Full Text
    1. Perkins LA,
    2. Holderbaum L,
    3. Tao R,
    4. Hu Y,
    5. Sopko R,
    6. McCall K,
    7. Yang-Zhou D,
    8. Flockhart I,
    9. Binari R,
    10. Shim HS, et al.
    (2015) The transgenic RNAi project at harvard medical school: Resources and validation. Genetics 201: 843852. doi:10.1534/genetics.115.180208
    OpenUrlAbstract/FREE Full Text
    1. Perrimon N,
    2. Ni JQ,
    3. Perkins L
    (2010) In vivo RNAi: Today and tomorrow. Cold Spring Harb Perspect Biol 2: a003640. doi:10.1101/cshperspect.a003640
    OpenUrlAbstract/FREE Full Text
    1. Piccin A,
    2. Salameh A,
    3. Benna C,
    4. Sandrelli F,
    5. Mazzotta G,
    6. Zordan M,
    7. Rosato E,
    8. Kyriacou CP,
    9. Costa R
    (2001) Efficient and heritable functional knock-out of an adult phenotype in Drosophila using a GAL4-driven hairpin RNA incorporating a heterologous spacer. Nucleic Acids Res 29: E55E65. doi:10.1093/nar/29.12.e55
    OpenUrlCrossRefPubMed
    1. Pletcher RC,
    2. Hardman SL,
    3. Intagliata SF,
    4. Lawson RL,
    5. Page A,
    6. Tennessen JM
    (2019) A genetic screen using the Drosophila melanogaster TRiP RNAi collection to identify metabolic enzymes required for eye development. G3 (Bethesda) 9: 20612070. doi:10.1534/g3.119.400193
    OpenUrlAbstract/FREE Full Text
    1. Port F,
    2. Hausmann G,
    3. Basler K
    (2011) A genome-wide RNA interference screen uncovers two p24 proteins as regulators of Wingless secretion. EMBO Rep 12: 11441152. doi:10.1038/embor.2011.165
    OpenUrlAbstract/FREE Full Text
    1. Reece-Hoyes JS,
    2. Walhout AJM
    (2018) Gateway recombinational cloning. Cold Spring Harb Protoc 2018: top094912. doi:10.1101/pdb.top094912
    OpenUrlCrossRef
    1. Rotelli MD,
    2. Bolling AM,
    3. Killion AW,
    4. Weinberg AJ,
    5. Dixon MJ,
    6. Calvi BR
    (2019) An RNAi screen for genes required for growth of Drosophila wing tissue. G3 (Bethesda) 9: 30873100. doi:10.1534/g3.119.400581
    OpenUrlAbstract/FREE Full Text
    1. Rubin GM,
    2. Spradling AC
    (1982) Genetic transformation of Drosophila with transposable element vectors. Science 218: 348353. doi:10.1126/science.6289436
    OpenUrlAbstract/FREE Full Text
    1. Rust K,
    2. Tiwari MD,
    3. Mishra VK,
    4. Grawe F,
    5. Wodarz A
    (2018) Myc and the Tip60 chromatin remodeling complex control neuroblast maintenance and polarity in Drosophila. EMBO J 37: e98659. doi:10.15252/embj.201798659
    OpenUrlCrossRef
    1. Rylee J,
    2. Mahato S,
    3. Aldrich J,
    4. Bergh E,
    5. Sizemore B,
    6. Feder LE,
    7. Grega S,
    8. Helms K,
    9. Maar M,
    10. Britt SG, et al.
    (2022) A TRiP RNAi screen to identify molecules necessary for Drosophila photoreceptor differentiation. G3 (Bethesda) 12: jkac257. doi:10.1093/g3journal/jkac257
    OpenUrlCrossRef
    1. Saj A,
    2. Arziman Z,
    3. Stempfle D,
    4. van Belle W,
    5. Sauder U,
    6. Horn T,
    7. Dürrenberger M,
    8. Paro R,
    9. Boutros M,
    10. Merdes G
    (2010) A combined ex vivo and in vivo RNAi screen for notch regulators in Drosophila reveals an extensive notch interaction network. Dev Cell 18: 862876. doi:10.1016/j.devcel.2010.03.013
    OpenUrlCrossRefPubMed
    1. Santos-Pereira JM,
    2. Aguilera A
    (2015) R loops: New modulators of genome dynamics and function. Nat Rev Genet 16: 583597. doi:10.1038/nrg3961
    OpenUrlCrossRefPubMed
    1. Sarov M,
    2. Schneider S,
    3. Pozniakovski A,
    4. Roguev A,
    5. Ernst S,
    6. Zhang Y,
    7. Hyman AA,
    8. Stewart AF
    (2006) A recombineering pipeline for functional genomics applied to Caenorhabditis elegans. Nat Methods 3: 839844. doi:10.1038/nmeth933
    OpenUrlCrossRefPubMed
    1. Tomari Y,
    2. Zamore PD
    (2005) Perspective: Machines for RNAi. Genes Dev 19: 517529. doi:10.1101/gad.1284105
    OpenUrlAbstract/FREE Full Text
    1. van der Graaf K,
    2. Srivastav S,
    3. Singh P,
    4. McNew JA,
    5. Stern M
    (2022) The Drosophila attP40 docking site and derivatives are insertion mutations of MSP300. BioRxiv doi:10.1101/2022.05.14.491875 (Preprint posted May 15, 2022).
    OpenUrlAbstract/FREE Full Text
    1. Vissers JH,
    2. Manning SA,
    3. Kulkarni A,
    4. Harvey KF
    (2016) A Drosophila RNAi library modulates Hippo pathway-dependent tissue growth. Nat Commun 7: 10368. doi:10.1038/ncomms10368
    OpenUrlCrossRefPubMed
    1. Wargelius A,
    2. Ellingsen S,
    3. Fjose A
    (1999) Double-stranded RNA induces specific developmental defects in zebrafish embryos. Biochem Biophys Res Commun 263: 156161. doi:10.1006/bbrc.1999.1343
    OpenUrlCrossRefPubMed
    1. Wianny F,
    2. Zernicka-Goetz M
    (2000) Specific interference with gene function by double-stranded RNA in early mouse development. Nat Cell Biol 2: 7075. doi:10.1038/35000016
    OpenUrlCrossRefPubMed
    1. Zamore PD,
    2. Tuschl T,
    3. Sharp PA,
    4. Bartel DP
    (2000) RNAi: Double-stranded RNA directs the ATP-dependent cleavage of mRNA at 21 to 23 nucleotide intervals. Cell 101: 2533. doi:10.1016/s0092-8674(00)80620-0
    OpenUrlCrossRefPubMed
    1. Zeng X,
    2. Han L,
    3. Singh SR,
    4. Liu H,
    5. Neumuller RA,
    6. Yan D,
    7. Hu Y,
    8. Liu Y,
    9. Liu W,
    10. Lin X, et al.
    (2015) Genome-wide RNAi screen identifies networks involved in intestinal stem cell regulation in Drosophila. Cell Rep 10: 12261238. doi:10.1016/j.celrep.2015.01.051
    OpenUrlCrossRefPubMed
    1. Zhou J,
    2. Xu L,
    3. Duan X,
    4. Liu W,
    5. Zhao X,
    6. Wang X,
    7. Shang W,
    8. Fang X,
    9. Yang H,
    10. Jia L, et al.
    (2019) Large-scale RNAi screen identified Dhpr as a regulator of mitochondrial morphology and tissue homeostasis. Sci Adv 5: eaax0365. doi:10.1126/sciadv.aax0365
    OpenUrlFREE Full Text
    1. Zielke N,
    2. Korzelius J,
    3. van Straaten M,
    4. Bender K,
    5. Schuhknecht GFP,
    6. Dutta D,
    7. Xiang J,
    8. Edgar BA
    (2014) Fly-FUCCI: A versatile tool for studying cell proliferation in complex tissues. Cell Rep 7: 588598. doi:10.1016/j.celrep.2014.03.020
    OpenUrlCrossRefPubMed
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Drosophila pVALIUM10 TRiP RNAi lines found their off-targets
Dimitrije Stanković, Gábor Csordás, Mirka Uhlirova
Life Science Alliance Nov 2022, 6 (2) e202201801; DOI: 10.26508/lsa.202201801
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