Abstract
Mobile group II introns are bacterial retrotransposons that are thought to have invaded early eukaryotes and evolved into introns and retroelements in higher organisms. In bacteria, group II introns typically retrohome via full reverse splicing of an excised intron lariat RNA into a DNA site, where it is reverse transcribed by the intron-encoded protein. Recently, we showed that linear group II intron RNAs, which can result from hydrolytic splicing or debranching of lariat RNAs, can retrohome in eukaryotes by performing only the first step of reverse splicing, ligating their 3′ end to the downstream DNA exon. Reverse transcription then yields an intron cDNA, whose free end is linked to the upstream DNA exon by an error-prone process that yields junctions similar to those formed by non-homologous end joining (NHEJ). Here, by using Drosophila melanogaster NHEJ mutants, we show that linear intron RNA retrohoming occurs by major Lig4-dependent and minor Lig4-independent mechanisms, which appear to be related to classical and alternate NHEJ, respectively. The DNA repair polymerase θ plays a crucial role in both pathways. Surprisingly, however, mutations in Ku70, which functions in capping chromosome ends during NHEJ, have only moderate, possibly indirect effects, suggesting that both Lig4 and the alternate end-joining ligase act in some retrohoming events independently of Ku. Another potential Lig4-independent mechanism, reverse transcriptase template switching from the intron RNA to the upstream exon DNA, occurs in vitro, but gives junctions differing from the majority in vivo. Our results show that group II introns can utilize cellular NHEJ enzymes for retromobility in higher organisms, possibly exploiting mechanisms that contribute to retrotransposition and mitigate DNA damage by resident retrotransposons. Additionally, our results reveal novel activities of group II intron reverse transcriptases, with implications for retrohoming mechanisms and potential biotechnological applications.
Author Summary
Group II introns are bacterial mobile elements thought to be ancestors of introns and retrotransposons in higher organisms. They consist of a catalytically active intron RNA and an intron-encoded reverse transcriptase, which function together to promote intron integration into new DNA sites in a process called “retrohoming.” In bacteria, retrohoming occurs by the excised intron lariat RNA fully reverse splicing into a DNA site, where it is reverse transcribed, yielding an intron cDNA that is copied directly into the host genome. However, little is known about how group II introns behave in higher organisms. Here, we find that linear group II intron RNAs, which cannot fully reverse splice, retrohome in Drosophila melanogaster by attaching themselves to only one end of a DNA site. Reverse transcription then yields an intron cDNA, which is integrated into the recipient DNA by host enzymes that function in non-homologous end joining, a critical cellular DNA–repair pathway. Biochemical experiments exploring alternate mechanisms show that group II intron reverse transcriptases can also template switch efficiently from one RNA template to a second RNA or DNA template, thereby directly linking the two template sequences. Our findings have implications for retotransposition and DNA repair mechanisms and potential biotechnological applications.
Introduction
Mobile group II introns are site-specific retrotransposons that consist of a catalytically active intron RNA (ribozyme) and an intron-encoded protein (IEP), with reverse transcriptase (RT) activity [1]. Although they are found mainly in bacterial and organellar genomes, group II introns are thought to have played a major role in eukaryotic genome evolution as evolutionary ancestors of nuclear spliceosomal introns and retrotransposons in higher organisms [2]–[4]. Group II intron RNAs catalyze their own splicing via two sequential transesterification reactions that are the same as those for spliceosomal introns and yield an excised intron lariat with a branched 2′-5′ phosphodiester linkage [5], [6]. For mobile group II introns, the splicing reactions are assisted by the IEP, which binds specifically to the intron RNA and stabilizes the catalytically active RNA structure [7], [8]. The IEP then remains bound to the excised intron lariat RNA in a ribonucleoprotein particle (RNP) that promotes intron integration into new DNA sites [9], [10]. Intron integration is targeted to the ligated-exon junction in an intronless alleles in a process called “retrohoming”, but can also occur at lower frequency into ectopic sites that resemble the homing site in a process called “retrotransposition” or “ectopic retrohoming”. In both cases, the intron inserts into the new DNA site by a novel mechanism in which the excised intron lariat RNA fully reverse splices into a DNA strand and is reverse transcribed by the IEP, yielding an intron cDNA that is integrated into the genome by host enzymes [1], [10]–[14]. Retrohoming leads to the expansion of intron-containing alleles in a population, while ectopic retrohoming provides a means of intron dispersal to new sites.
Group II intron RNAs can also splice without branching by an alternate pathway, termed “hydrolytic splicing” [1]. In this pathway, the first transesterification, 5′-splice site cleavage, occurs by hydrolysis rather than branching, and the second transesterification yields ligated exons and an excised linear intron RNA. Hydrolytic splicing was first observed as a side reaction of group II intron self-splicing under non-physiological conditions [15], [16] and was demonstrated to occur in vivo by using a mutant yeast mitochondrial intron that was deleted for the branch-point A residue [17]. Some subclasses of group II introns lack the branch-point A residue and rely entirely on the hydrolytic mechanism for splicing in vivo [18], [19]. Linear group II intron RNAs can also be generated from excised intron lariat RNAs by debranching, which is believed to accelerate RNA turnover [20]. However, the physiological and evolutionary significance of hydrolytic splicing and linear group II intron RNAs have remained largely unclear.
The Lactococcus lactis Ll.LtrB intron, which has been used extensively as a model system for studying group II intron mobility mechanisms, has a broad host range and is actively mobile in Escherichia coli, making it possible to use E. coli genetic approaches to dissect mobility pathways [11], [21]. The major retrohoming pathway used by the Ll.LtrB intron in E. coli is shown in Figure 1A. After promoting splicing, the Ll.LtrB IEP, denoted LtrA protein, remains bound to the excised intron lariat RNA in RNPs that recognize a DNA target site at the ligated-exon junction (denoted E1–E2) of an intronless allele. The intron lariat RNA initiates retrohoming by fully reverse splicing into the top DNA strand, leading to insertion of the intron RNA between the two DNA exons. The IEP then uses a DNA endonuclease activity to cleave the bottom strand and uses the 3′ DNA end at the cleavage site as a primer for reverse transcription of the inserted intron RNA. In E. coli, the resulting intron cDNA is integrated into the host genome by a mechanism that involves degradation of the intron RNA template strand by a host RNase H and second-strand DNA synthesis by a host DNA polymerase [11], [21]. In variations of this mechanism, Ll.LtrB and other group II introns can also retrohome without bottom-strand DNA cleavage by using a nascent strand at a DNA replication fork to prime reverse transcription of the intron RNA [14], [22], [23], and yeast mitochondrial group II introns retrohome by using recombination rather than DNA repair for cDNA integration [24].
Recently, while carrying out experiments to test whether microinjected group II intron RNPs could be used for gene targeting in Xenopus laevis oocyte nuclei and Drosophila melanogaster embryos, we found that linear as well as lariat group II intron RNAs can retrohome in vivo [25]. This finding was surprising because, unlike lariat RNAs, linear group II intron RNAs can carry out only the first reverse-splicing step, ligation of the 3′ end of the intron RNA to the 5′ end of the 3′- exon DNA [26], [27]. While reverse transcription of fully reverse-spliced intron RNA yields an intron cDNA that can be extended directly by continued DNA synthesis into the upstream exon (Figure 1A), reverse transcription of a partially reverse-spliced intron RNA yields an intron cDNA with an unattached 3′ end that must be linked to the upstream exon DNA in a separate step (Figure 1B). Sequencing of 5′-integration junctions showed that this step occurs by an error-prone process. Although some events result in the precise insertion of the intron between the two DNA exons, most give 5′-integration junctions with 5′-exon deletions, intron 5′-end truncations, insertion of extra nucleotides at the intron-exon junction, or indications of DNA repair via base pairing of microhomologies on opposite sides of the break [25], similar to ligation junctions resulting from double-strand break repair by non-homologous end joining (NHEJ) [28]–[31]. NHEJ activities have been found to contribute to the retrotransposition of LINE elements and other retrotransposons in eukaryotes [32], [33] and may be exploited preferentially by retrotransposons to gain advantage in genetic conflict with their hosts, which rely on these enzymes for survival [34]. Thus, although group II introns are alien to Xenopus and Drosophila, they could be utilizing mechanisms that contribute to the retrotransposition of resident retroelements in eukaryotes and could be subject to host defenses that evolved to counter or mitigate such retrotransposition.
Although NHEJ seemed the most likely mechanism for attachment of the free cDNA to the 5′ exon in linear intron RNA retrohoming, an alternate possibility was that the RT template switches to the 5′-exon DNA, either directly or following incorporation of extra nucleotide residues at the end of the cDNA, resulting in synthesis of a continuous DNA bottom strand containing intron and 5′-exon sequences. Both template switching and incorporation of extra nucleotide residues at the ends of cDNA have been found for other non-LTR-retroelement RTs [35]–[37]. Although we thought this possibility unlikely because group II intron RTs appeared to have low DNA-dependent DNA polymerase activity in vitro [21], template switching and non-templated nucleotide addition by group II intron RTs have not been investigated previously.
Here, we used Drosophila melanogaster mutants to investigate the contribution of NHEJ activities to linear intron RNA retrohoming and assessed the involvement of template switching by comparing junctions formed by this mechanism in vitro with those formed during linear intron RNA retrohoming in vivo. Our results indicate that linear intron RNA retrohoming occurs primarily by a novel variation of NHEJ that uses host enzymes, including DNA ligase 4 (Lig4) and DNA repair polymerase θ (PolQ), but is minimally dependent upon Ku.
Results
Retrohoming of linear and lariat RNA in D. melanogaster mutant embryos
To investigate the involvement of NHEJ factors, we compared lariat and linear group II intron retrohoming in D. melanogaster embryos with mutations in the genes encoding DNA ligase 4 (Lig4), Ku70, and the DNA repair polymerase θ (PolQ) [38], [39]. For these experiments, we used a plasmid-based retrohoming assay in which an Ll.LtrB-ΔORF intron with a phage T7 promoter sequence inserted near its 3′ end integrates into a target site cloned in an AmpR-recipient plasmid upstream of a promoterless tet R reporter gene, thereby activating that gene (Figure 2A) [25], [26], [40]. The recipient plasmid was injected into the posterior of precellular blastoderm stage embryos, followed within 5 min by injection of lariat or linear RNPs, which were reconstituted in vitro from the purified IEP and intron RNA (see Materials and Methods). After incubating the embryos for 1 h at 30°C, nucleic acids were extracted and transformed into an E. coli strain (HMS174(DE3)), which expresses T7 RNA polymerase. The transformed bacteria were then plated on medium containing ampicillin or ampicillin and tetracycline, and mobility efficiencies were quantified as the ratio of (TetR+AmpR)/AmpR colonies.
Figure 2B compares the retrohoming efficiencies of lariat and linear intron RNAs in wild-type and mutant embryos, based on parallel assays in ten separate experiments (summarized in Table S1). For each strain in each experiment, 80 injected embryos were pooled prior to extracting nucleic acids and transforming them into E. coli. The results for the lig4 mutant show the retrohoming efficiency of the lariat intron was unchanged, whereas the retrohoming efficiency of the linear intron was decreased strongly (18% wild type), but could be restored to wild-type levels by ectopic expression of Lig4 from an integrated P-element (lig4−; P{lig4+} embryos). In the polQ mutant, the retrohoming efficiency of the linear intron was decreased to ≤0.5% of wild type, compared to 27% wild type for lariat RNPs. Finally, the ku70 mutant, a trans-heterozygote of two putative null alleles (see Materials and Methods), showed only moderately decreased retrohoming efficiencies for both lariat and linear intron retrohoming (67% and 46% wild type, respectively). The latter result was surprising because Ku and Lig4 ordinarily function together in the same NHEJ pathway [41], [42].
The strong differential inhibition of linear compared to lariat RNA retrohoming in the lig4 and polQ mutants supports models in which these enzymes function directly at unique steps in this process, presumably by providing the DNA ligase and repair DNA polymerase activities needed to link the intron cDNA to the upstream exon. The similar moderate decreases in lariat and linear intron retrohoming efficiency in the ku70 mutant could reflect that Ku functions at a common step in both pathways or could be an indirect effect (see Discussion).
Comparison of 5′-integration junctions from linear intron RNA retrohoming in wild-type and lig4 and ku70 mutant embryos
D. melanogaster uses at least two NHEJ pathways to repair double-strand breaks: classical NHEJ (C-NHEJ), which is dependent upon Lig4 and Ku70, and alternate end-joining (alt-EJ), which operates without either factor and could be a mixture of different pathways [31], [38], [39], [43]. In a genetic assay for repair of double-strand breaks induced in the germline by the meganuclease I-SceI, lig4 and ku70 mutants inhibited NHEJ activity by 76–78%, leaving 22–24% residual activity that was attributed to alt-EJ [43]. Our finding above that the lig4 mutant shows similar degrees of inhibition and residual activity for linear intron retrohoming (82% and 18%, respectively), most simply suggests that Lig4-independent retrohoming occurs by using the alt-EJ pathway or components thereof.
Previous studies showed that the DNA repair junctions resulting from alt-EJ in Drosophila ku70 and lig4 mutants are generally similar to those for C-NHEJ [31], although in some assays, the lig4 mutant gave somewhat increased frequencies of junctions with extra nucleotide additions (55–63% compared to 30–36% for wild type [38], [39]). To further investigate whether Lig4-independent retrohoming occurs via alt-EJ, we compared 5′- and 3′-intron integration junctions resulting from linear intron retrohoming in the mutant and two commonly used wild-type strains (w1118 and Or-R) by PCR using primers flanking the junctions, followed by cloning and sequencing of the PCR products (Figure 3 and Figure 4).
The 5′- and 3′-integration junctions from lariat intron retrohoming and the 3′-integration junctions from linear intron retrohoming result from reverse-splicing reactions (see Figure 1), and as expected, the PCRs for these junctions gave single prominent products, with no differences between the wild-type and mutant strains (Figure 3, bottom gels; in each case, the expected precise junction sequence was confirmed by sequencing; see legend for details). By contrast, the 5′-integration junctions resulting from linear intron RNA retrohoming were heterogeneous in all strains, with a major band of the size expected for full-length intron insertion and smaller bands, which appeared most prominent in the lig4−; P{lig4+} and polQ − embryos (Figure 3, top gels).
DNA sequences of the 5′-integration junctions resulting from linear intron retrohoming in wild-type w1118 and lig4−, ku70−, and lig4−; P{lig4+} embryos are summarized in Figure 4A–4D, and their characteristics are compared by the bar graphs in Figure 5. As found previously [25], the 5′-integration junctions for linear intron RNA retrohoming in the wild-type embryos were heterogeneous with different combinations of 5′-exon deletions, 5′-intron truncations, and extra nucleotide additions (Figure 4A). Some of the junctions show evidence of DNA repair at regions of microhomology (parentheses), and in some cases, the extra nucleotides inserted at the junctions match and were presumably copied from neighboring sequences in the 5′ exon or intron (underlined).
The 5′ junctions resulting from linear intron retrohoming in the lig4 −, ku70 −, and lig4−; P{lig4+} mutants were generally similar to those in the wild type w1118, the more closely related wild-type strain, with no large differences in the percentage of junctions with 5′-exon deletions, 5′-intron truncations, extra nucleotide additions, or microhomologies (Figure 4 and Figure 5). Compared to the other strains assayed in parallel, the proportion of long 5′-intron truncations appears to be somewhat lower in the ku70− embryos and higher in the lig4 − and lig4−; P{lig4+} embryos, but the significance of these findings is unclear, as the differences were not large and the proportions of full-length and shorter 5′-junction products in each stock were somewhat variable in different experiments. The similarity of the junction sequences resulting from linear intron RNA retrohoming in the lig4 and ku70 mutants to those resulting from double-strand break repair in these mutants [31], [39] supports the hypothesis that Lig4-independent linear intron retrohoming occurs predominantly by using components of the alt-EJ pathway.
The polQ mutation decreases extra nucleotide addition and increases long microhomologies at 5′-integration junctions
The DNA repair polymerase θ (PolQ) has been shown to function in DNA end-joining repair in Drosophila, including a role for extra nucleotide addition at the repaired junctions [38]. To investigate the function of PolQ in linear intron RNA retrohoming, we compared the sequences of 5′-intregration junctions from parallel assays of this process in wild-type Or-R and polQ− embryos (Figure 4E and 4F, Figure 5). Because the number of unique junction sequences recovered from the polQ mutant was lower than those for the other strains and some of these junctions were represented multiple times, we calculated the proportion of junctions with different characteristics in Figure 5 relative to both the total number of junctions (left bars) and the total number of unique junctions sequences (right bars, asterisks). Both comparisons show that that the polQ mutation decreases the proportion of junctions containing extra nucleotide residues (4% of total junctions and 20% of unique junctions compared to >64% of junctions in wild-type Or-R and >48% in all other strains analyzed), as expected from the known function of PolQ. Further, the 5′ junctions from the polQ − embryos have a higher frequency of long (≥15 bp) 5′-exon deletions (72% of total junctions and 80% of unique junctions compared to 29% in wild-type Or-R) and a dramatically increased frequency of long (≥5 nt) microhomologies between exon and intron sequences (56% of total junctions and 40% of unique junctions compared to none among 170 total junctions from all the other strains analyzed). This increased frequency of long microhomologies may reflect that they are more stringently required for annealing of the 3′ end of the cDNA to the upstream exon in the absence of PolQ. We note that among the unique junction sequences from the polQ mutant, two with large deletions were recovered ≥10 times each. Although we cannot exclude that the repeated recovery of these junctions reflects differential amplification by PCR, both have ≥5 nt microhomologies that could have been used preferentially for annealing in multiple events, and indeed one of these junctions (Figure 4F bottom sequence) comprised 6 of 12 recovered junctions in an additional, separate experiment (data not included in Figure 4F). Considered together, the junction sequences indicate that PolQ functions in extra nucleotide addition to the 3′ end of the cDNA during linear intron RNA retrohoming and that this extra nucleotide addition may be critical for generating microhomologies that enable annealing between the 3′ end of the cDNA and the upstream exon DNA. Further, the strongly decreased frequency of linear intron RNA retrohoming in the polQ mutant indicates that PolQ functions in both the Lig4-dependent and Lig4-independent retrohoming pathways.
The Ll.LtrB RT can template switch from the 5′ end of linear intron RNA to the upstream exon
Although the residual linear intron RNA retrohoming events in the lig4 mutant can be accounted for by Lig4-independent (alt-EJ) NHEJ, it remained possible that template switching of the RT from the 5′ end of the intron RNA directly to the 3′ end of the 5′-exon DNA contributes to this process. Previous studies have shown that other non-LTR retroelement RTs are proficient at template switching directly to the 3′ end of a template strand with little or no complementarity to the cDNA end and that these events can be accompanied by extra nucleotide addition at the junctions, as found for NHEJ [35], [36], [37], [44].
To determine if a template-switching mechanism could be responsible for the manner of 5′ junctions observed during linear intron retrohoming, we carried out biochemical assays using small artificial substrates that simulate the situation at the 5′-integration junction just prior to completion of intron cDNA synthesis (Figure 6). The primary substrate consists of a 60-nt RNA template (Ll.LtrB RNA), whose 5′ end corresponds to that of the Ll.LtrB intron, with a 45-nt DNA primer representing the nascent cDNA (primer c) annealed to its 3′ end. The Ll.LtrB RT (LtrA) initiates reverse transcription of the intron RNA template from the annealed DNA primer and extends it to the 5′ end of the Ll.LtrB RNA template, where it can then switch to a second 40-nt DNA or RNA template with the nucleotide sequence of exon 1 (E1 RNA or DNA, red and black, lanes 5 and 6, respectively). The 3′ end of the Ll.LtrB RNA has an aminoblock to impede the RT from switching to a second molecule of the initial template.
Figure 6, lanes 5 and 6 show that the Ll.LtrB RT efficiently extends the annealed primer c (Pri c) to the end of the intron RNA template, yielding major labeled products of ∼60-nt, which were resolved as a doublet, along with smaller amounts of larger products of the size expected for template switching to the exon 1 (E1) DNA or RNA (∼100 nt) or to a second molecule of Ll.LtrB RNA despite the presence of the aminoblock (∼120 nt). Controls show that no labeled products were detected after incubating the RT with primer c in the presence or absence of the exon 1 RNA or DNA (lanes 2–4).
Cloning and sequencing of the gel bands confirmed that the major ∼60-nt products (bands a and b in lane 5 and h and i in lanes 6) correspond to cDNAs extending to or near the 5′ end of the intron RNA, with the doublet reflecting the addition of extra nucleotide residues, mostly A-residues, to the 3′ end of the cDNA upon reaching the end of the Ll.LtrB RNA template (Figure 7A and 7B). Such non-templated nucleotide addition is a common property of DNA polymerases and RTs [35], [36], [45]–[48].
The first set of larger gel bands (90–110 nts; band c–e in lane 5 and j–l in lane 6) corresponds to products resulting from template switching from the 5′ end of the intron to the 3′ end of exon 1 DNA or RNA (Figure 7A and 7B), as well as products resulting from template switching to the 3′ end or internal regions of the Ll.LtrB intron (Figure S1). Many of the template switches to exon 1 DNA occurred seamlessly, but small numbers of extra nucleotide residues, mostly A residues, were found at some junctions, as well as at the 3′ end of the cDNAs (Figure 7A; bands c–e). The template switches to exon 1 RNA showed similar characteristics, but with a higher proportion of junctions containing extra nucleotide residues (61% compared to 33% for exon 1 DNA; Figure 7B; bands j–l).
The second set of larger bands (120–140 nts; bands f and g in lane 5 and m and n in lane 6) contains products resulting from two sequential template switches to exon 1 DNA or RNA (Figure 7A and 7B, respectively) and/or the Ll.LtrB RNA (Figure S1). These products of multiple template switches have characteristics similar to those resulting from a single template switch, including addition of extra nucleotide residues, mostly A residues, at some template-switching junctions and at the 3′ ends of the cDNAs.
The above results were obtained under reaction optimized for reverse transcription by the Ll.LtrB RT in vitro (450 mM NaCl, 5 mM Mg2+), the high salt concentration helping to stabilize free protein and minimize aggregation of this RT [9]. However, similar results were obtained for template-switching reactions under near-physiological salt conditions (100 or 200 mM KCl, 5 mM Mg2+). Although the RT activity of the protein was lower under these conditions, the gel profiles show roughly equal levels of template switching to exon 1 RNA and DNA (Figure S2), and sequencing of the products showed similar template-switching junctions and patterns of non-templated nucleotide addition (Figure S3).
Finally, we tested whether the Ll.LtrB RT could template switch to double-stranded exon 1 DNA or RNA with an annealed bottom-strand DNA leaving either a blunt end or a 5′ bottom-strand overhang identical to that generated in vivo by the staggered double-strand break accompanying group II intron insertion (Figure 1; complete annealing confirmed by native gel analysis; Figure S4). Neither of these configurations significantly decreased the formation of the 100-nt product resulting from template switching to exon 1 DNA or RNA (Figure 6, lanes 7–9). DNA sequencing confirmed the template switch to double-stranded E1 DNA with a 5′-bottom-strand overhang and showed that this template switch was seamless in most cases (Figure 7C). The sequencing also showed several instances in which the template switch occurred to the penultimate rather than the 3′ terminal residue of exon 1 (Figure 7C), as well as template switches to Ll.LtrB RNA and the bottom-strand overhang oligonucleotide (Figure S5). Template switching to the penultimate nucleotide residue was not seen for single-strand acceptor DNA templates and could be related to the presence of the complementary DNA strand.
Together, the biochemical assays show that the Ll.LtrB RT can template switch from the 5′ end of the intron RNA to exon 1 and surprisingly that template switching is similarly efficient regardless of whether the exon 1 template is RNA or DNA or single- or double-stranded. However, the junctions resulting from template switching differ from those generated during retrohoming of linear intron RNA in vivo in that extra nucleotide additions are uniformly short and mostly A-residues.
Discussion
Considered together, our results lead to the model shown in Figure 8 for the key steps in linear intron RNA retrohoming. The finding of strong differential inhibition of linear relative to lariat intron retrohoming in D. melanogaster mutants indicates that the NHEJ factor Lig4 is the predominant enzyme involved in ligating the intron cDNA to the upstream exon and that extra nucleotide addition by the DNA repair polymerase θ (PolQ) also plays a crucial role. Although Lig4 and PolQ appear to be the major enzymes playing these roles in D. melanogaster, residual linear intron RNA retrohoming with extra nucleotide addition occurs in both the lig4 and polQ mutants, indicating that other DNA ligases and polymerases can serve as backups that perform the same functions at lower efficiency. Biochemical experiments show that another possible Lig4-independent mechanism, template switching by the group II intron RT from the 5′ end of the intron RNA directly to the upstream exon DNA, is possible but gives junctions differing from the majority of those in vivo. It seems likely that the mechanism elucidated here involving host DNA ligases and repair polymerases is also used for linear intron RNA retrohoming in Xenopus laevis, where we observed similar 5′-integration junctions [25], and more generally, in other eukaryotes, including mammalian cells, where it could have implications for group II intron-based gene targeting. This mechanism also provides a possible means for proliferation of non-branching group II introns in prokaryotes, some of which encode a Ku homolog and ATP-dependent DNA ligases along with DNA repair polymerases and use them in NHEJ pathways related to those of higher organisms [49]. Additionally, features of this mechanism, including the use of both Lig4-dependent and alt-EJ and the requirement for extra nucleotide addition to the cDNA end by a DNA repair polymerase, may be used to promote retrotransposition and mitigate DNA damage caused by LINE elements and other retrotransposons [33], [50]–[52].
The involvement of Lig4 in linear intron RNA retrohoming in Drosophila is indicated by the findings that a lig4 mutation decreases the retrohoming efficiency of linear intron RNA by ∼80% while having no effect on the retrohoming of lariat RNA, and that the decreased retrohoming efficiency of the linear intron in the mutant could be restored to wild-type levels by ectopic expression of Lig4 from a P-element insertion. Most if not all of the residual linear intron RNA retrohoming in the lig4 mutant appears to occur by using components of the alt-EJ pathway, as judged both by similar levels of activity and characteristics of the cDNA ligation junction, particularly patterns of extra nucleotide and the use of microhomologies (see Results). In Drosophila, C-NHEJ and alt-EJ give generally similar double-strand break repair junctions, albeit with quantitative differences in the frequency of extra nucleotide addition in some assays [31], [38], [39], whereas in yeast or mammalian cells, alt-EJ junctions show increased deletion lengths and use of microhomologies [53]–[55].
The involvement of PolQ in linear intron RNA retrohoming is indicated by the findings that a PolQ mutation decreases the retrohoming efficiency by >99% and substantially decreases the frequency of 5′-integration junctions having extra nucleotide residues (4–20% of junctions compared to 67% for wild-type Or-R assayed in parallel and >48% in all other strains; Figure 4 and Figure 5). The mutation also increases the frequency of junctions with long (≥15 bp) 5′-exon deletions and long (≥5 nt) microhomologies. The latter increase is particularly striking, as such long microhomologies were found at 56% of the total and 40% of the unique junction sequences from the polQ mutant, but were not found at junctions (170 total) from any of the other strains analyzed (Figure 4 and Figure 5). The residual extra nucleotide addition in the polQ mutant, which was also seen at 15–20% of junctions in end-joining assays [38], [39], could be due to small amounts of the enzyme remaining in the mutant, which has an unidentified expression defect, or to an alternate DNA polymerase. The very strong decrease in linear intron RNA retrohoming efficiency in the polQ mutant (>99%) indicates that PolQ functions in both the Lig4-dependent and Lig4-independent retrohoming pathways.
PolQ could potentially play at least two roles in linear intron RNA retrohoming. First, extra nucleotide addition to the 3′ end of the cDNA by PolQ may be critical for generating microhomologies that can base pair with the upstream exon to facilitate DNA ligation. Second, PolQ contains a putative DNA helicase domain that could also contribute to retrohoming by promoting base pairing between microhomologies at the cDNA end and the upstream exon, either by annealing the cDNA end to complementary exon sequences or by unwinding the exon DNA strands, making the top strand more accessible to base pairing [38]. The increased frequency of long 5′-exon deletions in the polQ mutant may reflect a delay in cDNA attachment due to lack of suitable microhomologies and/or impaired annealing of complementary cDNA ends to the top strand. The striking increase in the frequency of long microhomologies at the 5′ junctions in the polQ mutant (see above) indicates that an alternate annealing mechanism exists in the polQ mutants, but that it is more dependent upon longer microhomologies between exon and intron sequences than the PolQ-assisted mechanism.
The function, if any, of Ku in linear intron RNA retrohoming is unclear. The finding that ku70 mutations moderately inhibit retrohoming of both linear and lariat intron RNA (54 and 33% inhibition, respectively) could reflect either that Ku contributes to both pathways or that Ku mutations affect one or both pathways indirectly. The Ku protein interacts with a stem-loop region of the RNA component of yeast and human telomerase [56]–[58], and it is possible that Ku may similarly bind to linear or lariat group II intron RNAs to protect them from degradation and/or recruit other DNA repair enzymes to the site. An alternate possibility is that Ku affects retrohoming efficiency indirectly by contributing to the repair of double-strand breaks induced by the intron RNP in the recipient plasmids. In yeast mitochondria, double-strand breaks resulting from abortive retrohoming events are substantially more frequent than completed integrations [59]. If not repaired correctly, such double-strand breaks could lead to loss of functional recipient plasmid target sites, which would appear as decreased retrohoming efficiencies in our assay. A similar indirect effect, involving repair of double-strand breaks in the recipient plasmid could also account for the moderate inhibitory effect of the polQ mutation on lariat intron RNA retrohoming.
Lig4 is ordinarily recruited to DNA breaks by Ku, and D. melanogaster mutations in either lig4 or ku70 give similar decreases in NHEJ efficiency, suggesting that Lig4 acts exclusively in Ku-dependent NHEJ [41]–[43]. By contrast, we find that linear intron RNA retrohoming is more strongly inhibited by a lig4 mutation than by putative null mutations in ku70 (82 and 54% inhibition, respectively). Even assuming that the inhibition by the ku70 mutations is a direct effect, these findings most simply suggest that a substantial proportion of linear intron RNA retrohoming events are promoted by Lig4 in the absence of Ku.
Unlike a conventional double-strand break, the double-strand break formed during linear intron RNA retrohoming has an RNA attached to one of the DNA ends, and this difference could potentially affect the recruitment and use of NHEJ activities. We noted previously that group II intron RNPs bind to both the 5′- and 3′-exons during retrohoming, and such bridging of the ligation junction could impede access and decrease the need for Ku to cap the broken DNA ends [25]. Additionally, the attached intron RNA could contribute directly to the recruitment of NHEJ activities. The interaction of Ku with telomerase RNA noted above is thought to help recruit telomerase to double-strand breaks [57], and it is possible that a similar interaction between Ku and the attached group II intron RNA contributes to the recruitment of Lig4 for some linear intron RNA retrohoming events. More generally, such a mechanism involving the interaction of Ku with RNA could also be used by LINE elements and other retrotransposons to recruit Lig4 and other NHEJ activities for cDNA integration and repair of DNA breaks.
Finally, our biochemical experiments demonstrate that template switching by the group II intron RT from the 5′ end of the intron RNA directly to the 3′ end of the upstream DNA exon is a potential alternate mechanism for cDNA attachment during linear intron RNA retrohoming. Although we found previously that the Ll.LtrB RT has low DNA-dependent DNA polymerase activity in vitro [21], we find here that it template switches and copies 5′-exon DNA templates as well as 5′-exon RNA templates (Figure 6), possibly reflecting that reverse transcription favors a conformation of the enzyme that can initiate more efficiently on DNA templates. In many cases, the template-switching junctions to DNA or RNA templates are seamless, but some have a small number of extra nucleotide residues, predominantly A-residues (corresponding to T-residues in the top strand) that were added by the RT to the 3′ end of the cDNA prior to the template switch. This pattern of extra nucleotide addition, which we found under both enzyme optimal and near-physiological conditions, differs from the majority of 5′-integration junctions resulting from linear intron retrohoming in vivo, where the extra nucleotide residues do not show a similar bias and sometimes correspond to copies of neighboring DNA sequences. It remains possible, however, that template switching by the Ll.LtrB RT could give different junctions in vivo, and that template switching and extra nucleotide addition by this enzyme contributes to some retrohoming events. We note that the ability of the group II intron RT's template switching activity to efficiently link sequences in two different templates could potentially be used to directly attach linker sequences containing primer-binding sites to the ends of cDNAs for cDNA cloning and sequencing applications.
Materials and Methods
D. melanogaster stocks
Flies were raised in standard fly media at 22°C. The lig4169 mutant, obtained from Mitch McVey (Tufts University, Medford, MA), has a deletion that removes the start codon and most of the region encoding the ATPase and adenylation domains [31]. The ku707B2 and ku70Ex8 mutants were obtained from William Engels (University of Wisconsin, Madison, WI). The ku707B2 allele lacks 1,359 bp at the 3′ end of the 2,393-bp gene, including most of the DNA and Ku80-interaction domains [43]. The ku70Ex8 allele lacks at least 1 kb, including all of exon 1 and the start codon [43]. The ku707B2/ku70Ex8 genotype, generated by crosses between trans-heterozygous ku707B2/ku70Ex8 parents, is the same as that used previously to study double-strand break repair pathways [39], [43].
The mus308D2 stock [60] was obtained from the Drosophila Stock Center (Bloomington, IA). The mutation lies outside of the coding region and results in undetectable levels of PolQ protein expression [38].
To obtain transgenic flies harboring a lig4 rescue fragment, a 6-kb DNA segment containing the lig4 gene was amplified from w1118 genomic DNA by using the Expand High Fidelity PCR System (Roche Applied Science, Indianapolis, IN), with primers Lig4 F1 BamHI (5′-AAGAGGATCCAGTAGCTGTAGAAGCAGCCAAC) and Lig4 R1 XhoI 5′-AAGACTCGAGCAGCAGTTCCTCCGACATGAAG). This PCR product was inserted between BamHI and XhoI sites of the P-element transformation vector pCaSpeR4 [61], and transgenic flies were produced by GenetiVision (Houston, TX). A transgene insertion on chromosome 2 was recombined with lig4169 to generate the fly stock used in P{lig4+} rescue experiments.
Except for the trans-heterozygous ku707B2/ku70Ex8 embryos (see above), embryos used for microinjection were obtained from crosses between isogenic wild-type or homozygous mutant parents. For all stocks, precellular blastoderm embryos were collected in egg laying chambers in under 40 min, microinjected with recipient plasmids and group II intron RNPs, and incubated for 1 h at 30°C prior to DNA extraction.
Recombinant plasmids
pACD5C, which was used for synthesis of lariat and linear intron Ll.LtrB intron RNAs, is a derivative intron-donor plasmid pACD4C with a T7 promoter sequence inserted in the sense orientation at the SalI site in intron DIV [25], [62].
pBRR3-ltrB, the target plasmid for intron-integration assays, contains the Ll.LtrB intron homing site (ligated exon 1 and 2 sequences of the ltrB gene from positions −178 upstream to +91 downstream of the intron-insertion site) cloned upstream of a promoterless tetR gene in an AmpR pBR322-based vector [63].
pIMP-1P, used for expression of the LtrA protein for RNP reconstitution, contains the LtrA ORF cloned downstream of a tac promoter and Φ10 Shine-Dalgarno sequence in the expression vector pCYB2 (New England BioLabs, Ipswich, MA) [9]. LtrA is expressed from this plasmid as a fusion protein with a C-terminal tag containing an intein-linked chitin-binding domain, enabling LtrA purification via a chitin-affinity column, followed by intein-cleavage [9].
pMAL-LtrA, used for expression of the LtrA protein for biochemical assays, contains the LtrA ORF [64] cloned downstream of a tac promoter and Φ10 Shine-Dalgarno sequence between BamHI and HindIII of the protein-expression vector pMAL-c2t. The latter is a derivative of pMal-c2x (New England BioLabs, Ipswich MA) with a TEV protease-cleavage site in place of the factor Xa site [65]. LtrA is expressed from this plasmid with an N-terminal fusion to maltose-binding protein (MalE), enabling its purification via an amylose-affinity column, followed by TEV-protease cleavage to remove the tag (see below).
Preparation of Ll.LtrB lariat and linear RNAs
Ll.LtrB-ΔORF intron RNAs were transcribed from DNA templates generated by PCR of plasmid pACD5C with primers that append a phage T3 promoter sequence (underlined in sequences below) [26]. For the lariat precursor RNA, the PCR primers were pACD-T3 (5′-GGAGTCTAGAAATTAACCCTCACTAAAGGGAATTGTGAGCG) and NheIR (5′-CTAGCAGCACGCCATAGTGACTGGCG), and for linear intron RNA, the PCR primers were T3LIS-1G (5′-AATTAACCCTCACTAAAGTGCGCCCAGATAGGGTGTTAAGTCAAG) and HPLC-purified LtrB940a (5′-GTGAAGTAGGGAGGTACCGCCTTGTTC). The PCR products were purified by using the Wizard SV Gel and PCR Clean-up System (Promega), extracted with phenol-chloroform-isoamyl alcohol (phenol-CIA; 25∶24∶1 by volume), ethanol precipitated, and dissolved in nuclease-free water. In vitro transcription and the preparation of lariat and linear intron RNAs were as described [26].
Preparation of LtrA protein and RNPs
The LtrA protein used for RNP reconstitution was expressed in E. coli BL21(DE3) from the intein-based expression vector pImp-1P and purified via a chitin-affinity column and intein cleavage, as described [9], except that the column buffer contained 50 mM Tris-HCl, pH 8.0, 0.1 mM EDTA, and 0.1% NP-40. Ll.LtrB RNPs were reconstituted with the purified LtrA protein and in vitro-synthesized lariat or linear Ll.LtrB-ΔORF intron RNA, as described [26], except that the final RNP pellet was dissolved in 10 mM KCl, 5 mM MgCl2, and 40 mM HEPES, pH 8.0.
The LtrA protein used in biochemical assays was expressed in E. coli BL21(DE3) from the plasmid pMAL-LtrA. Cells were grown in starter cultures of LB medium overnight at 37°C, inoculated into 0.5-l LB medium in ultra-yield flasks, and autoinduced by growing at 37°C for 3 h, followed by 18°C for 24 h [66]. Cells were harvested by centrifugation (Beckman JLA-8.1000; 4,000× g, 15 min, 4°C), resuspended in 1 M NaCl, 20 mM Tris-HCl, pH 7.5, 20% glycerol, and 0.1 mg/ml lysozyme (Sigma-Aldrich, St. Louis, MO), kept on ice for 15 min, and lysed by 3 freeze-thaw cycles on dry ice followed by sonication (Branson 450 Sonifier, Branson Ultrasonics, Danbury, CT; three or four 10 sec bursts on ice at an amplitude of 60%, with 10 sec between bursts). After pelleting cell debris (Beckman JA-14 rotor, 10,000 rpm, 30 min, 4°C), nucleic acids were precipitated from the supernatant with 0.4% polyethylenimine (PEI) and constant stirring for 20 min at 4°C, followed by centrifugation (Beckman JA-14 rotor, 14,000 rpm, 30 min, 4°C). Proteins were precipitated from the supernatant by adding ammonium sulfate to 50% saturation with constant stirring for 1 h at 4°C. The precipitated proteins were pelleted (Beckman JA-14 rotor, 14,000 rpm, 30 min, 4°C), dissolved in 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol, and run through a 10-ml amylose column (FPLC; Amylose High-Flow resin; New England BioLabs, Ipswich, MA), which was washed with 3 column volumes of 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol and eluted with 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol containing 10 mM maltose. Fractions containing the MalE-LtrA fusion were incubated with TEV protease (80 µg/ml, 18 h, at 4°C), and imidazole was added to a final concentration of 40 mM. LtrA freed of the MalE tag was then purified by FPLC through a Ni-NTA equilibrated with 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol, 40 mM imidazole. The Ni-NTA column, which takes advantage of endogenous histidine residues in LtrA's C-terminal domain, was washed with 3 column volumes of 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol, 40 mM imidazole, and eluted in 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol, 300 mM imidazole. Finally, the peak LtrA fractions from the Ni-NTA column were further purified through two tandem 1-ml heparin Sepharose columns (New England BioLabs). The columns were equilibrated with 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol, loaded directly with LtrA protein from the Ni-NTA column, washed with 5-column volumes of 500 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol, and eluted with a 20-column volume gradient of 0.5 to 1 M NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol. The protein elutes approximately midway through the gradient at ∼750 mM NaCl. The purified protein was concentrated to 30 µM, exchanged into 100 mM NaCl, 20 mM Tris-HCl, pH 7.5, 10% glycerol by dialysis, flash-frozen in liquid nitrogen, and stored at −80°C.
Retrohoming assays and analysis of intron-integration junctions
Drosophila embryos were microinjected with ∼300 pl recipient plasmid pBRR3-ltrB at 1.4 mg/ml in solution with 500 mM MgCl2 and 17 mM dNTPs, followed within 5 min by ∼300 pl of Ll.LtrB lariat or linear RNPs at 2.6 mg/ml in 10 mM KCl, 5 mM MgCl2, 40 mM HEPES, pH 8.0. The RNPs consist of LtrA protein bound to Ll.LtrB lariat or linear intron RNA with a phage T7 promoter sequence inserted in intron domain IV, and the recipient plasmid contains the Ll.LtrB intron target site (ligated exon 1 and 2 sequences of the ltrB gene; E1 and E2) cloned upstream of a promoterless tet R gene in a pBR322-based vector carrying an AmpR marker. Site-specific integration of the intron into the target site introduces the T7 promoter upstream of the promoterless tet R gene, thereby activating that gene. Eighty embryos were injected and incubated at 30°C for 1 h for each assay. The pooled embryos were incubated in lysis buffer (20 mM Tris-HCl, pH 8.0, 5 mM EDTA, 400 mM NaCl, 1% SDS (w/v)) with 400 µg/ml proteinase K (Molecular Biology Grade; Sigma-Aldrich) for 1 h at 55°C, and then extracted with phenol-CIA. Nucleic acids were ethanol precipitated and dissolved in 12 µl of distilled water.
For assays of retrohoming efficiency, a 4-µl portion of the nucleic acid preparation was electroporated into electrocompetent E. coli HMS174(DE3) F−, hsdR, recA, rif r (Novagen, EMD Chemicals, Gibbstown, NJ), which expresses T7 RNA polymerase. Cells were plated at different dilutions on 2% agar containing LB medium with ampicillin (50 µg/ml) plus tetracycline (25 µg/ml) or the same concentration of ampicillin alone. Colonies were counted after overnight incubation at 37°C, and the integration efficiency was calculated as the ratio of (AmpR+TetR)/AmpR colonies.
For analysis of intron-integration junctions, a 1-µl portion of the nucleic acid preparation was used as template for PCR using Phusion High Fidelity PCR Master Mix with HF buffer (New England BioLabs). The 5′-junction PCRs were done with primers P1 (5′-CTGATCGATAGCTGAAACGC) and LtrB933a (5′-AGGGAGGTACCGCCTTGTTCACATTAC), and the 3′ junction PCRs were done with primers P3 (5′-CAGTGAATTTTTACGAACGAACAATAAC) and P4 (5′-AATGGACGATATCCCGCA). The PCR was done for 25 cycles for all strains, except for parallel assays of wild-type Or-R and the polQ mutant, which required 35 PCR cycles to obtain sufficient PCR product from the mutant. The PCR products were purified using a MinElute PCR purification Kit (Qiagen), cloned into a TOPO TA cloning vector (pCRII-TOPO; Invitrogen, Carlsbad, CA), and transformed into chemically competent E. coli (One Shot TOP10; Invitrogen). The cloned PCR products were then amplified from randomly picked colonies by colony PCR using Phusion High Fidelity PCR Master Mix with HF buffer and primers M13 F(-20) (5′- GTAAAACGACGGCCAGT) and M13 R(-26) (5′-CAGGAAACAGCTATGAC) for 25 cycles, and sequenced using primers M13 R(-24) (5′-GGAAACAGCTATGACCATG) or M13 F(-20) [67].
Biochemical assays of group II intron RT template switching
Biochemical assays were done by incubating purified LtrA protein (40 nM) with synthetic oligonucleotide substrates that correspond to the 5′ end of the Ll.LtrB intron (60-nt Ll.LtrB RNA; 40 nM) with an annealed 5′-32P-labeled DNA primer corresponding to nascent cDNA (45-nt Pri c; 44 nM) in the presence of exon 1 RNA or DNA (40-nt E1; 40 nM) in 20 µl of reaction medium containing 450 mM NaCl, 5 mM MgCl2, 20 mM Tris-HCl, pH 7.5, 1 mM dithiothreitol (DTT) and 200 µM dNTPs. The reaction components were assembled on ice with substrate added last and then incubated at 30°C for 30 min. Reactions were terminated by phenol-CIA extraction. Portions of the reaction product (3 µl) were added to an equal volume of gel loading buffer II (95% formamide, 18 mM EDTA and 0.025% each of SDS, xylene cyanol, and bromophenol blue; Ambion, Austin, TX), denatured at 98°C for 7 min, and analyzed by electrophoresis in a denaturing 10 or 15% polyacrylamide gel, which was visualized by scanning with a PhosphorImager (Typhoon Trio, GE Healthcare, Piscataway, NJ). 32P-labeled DNA products were excised from the gel, amplified by PCR, as described (Sabine Mohr, Scott Kuersten, and A.M.L., manuscript in preparation), and cloned into the TOPO-TA pCR2.1 vector (Invitrogen), according to the manufacturer's protocol. Random colonies were picked and the cloned PCR products were amplified by colony PCR using Phusion High Fidelity PCR Master Mix/HF buffer with primers M13 F(-20) and M13 R(-26), and sequenced using the M13 R(-24) primer (see above).
The oligonucleotides used in the biochemical assays were Ll.LtrB RNA [LtrB5'S20Anchor6,5 RNA] ((5′- GUGCGCCCAGAUAGGGUGUUCUCGUUGGCAAUGGUGUCCAACUUGUGCUGCCAGUGCUCG), with an aminoblock on its 3′ end); annealed primer c (5′- CGAGCACTGGCAGCACAAG-deoxyuridine-TGGACACCATTGCCAACGAGAACAC); and exon 1 DNA (5′-TGTGATTGCAACCCACGTCGATCGTGAACACATCCATAAC) or RNA (5′-UGUGAUUGCAACCCACGUCGAUCGUGAACACAUCCAUAAC). Oligonucleotides complementary to exon 1 DNA or RNA were: exon 1 AS (5′-GTTATGGATGTGTTCACGATCGACGTGGGTTGCAATCACA) and exon 1 AS+9 (5′-AATGATATGGTTATGGATGTGTTCACGATCGACGTGGGTTGCAATCACA).
DNA and RNA oligonucleotides used in the assays were obtained from Integrated DNA Technologies (IDT; Coralville, IA) and purified in a denaturing 10% (w/v) polyacrylamide gel. DNA primers were 5′-end labeled with [γ-32P]-ATP (10 Ci/mmol; Perkin-Elmer, Waltham, MA) by using phage T4 polynucleotide kinase (New England BioLabs) according to the manufacturer's protocol. Complementary oligonucleotides were annealed at ratios of 1∶1 (E1 oligonucleotides) or 1∶1.1 Ll.LtrB/primer c by mixing at 20 times the final concentration in annealing buffer (100 mM Tris-HCl, pH 7.5, and 5 mM EDTA), heating to 82°C, and slowly cooling to 25°C for 45 min. The efficiency of annealing was assessed by electrophoresis in a non-denaturing 6% polyacrylamide gel containing Tris-borate-EDTA (90 mM Tris, 90 mM boric acid, 2 mM EDTA) at 30°C [67].
Supporting Information
Acknowledgments
We thank Fanglei Zhuang and Sabine Mohr for helping design the group II intron reverse transcriptase template-switching experiments; Paul Macdonald and Janice Fischer for advice and use of equipment for D. melanogaster experiments; Mitch McVey (Tufts) and William Engels (University of Wisconsin) for fly stocks; and Paul Macdonald, Jacob Whitt, and Sabine Mohr for comments on the manuscript.
Footnotes
The authors have declared that no competing interests exist.
This work was supported by NIH grant GM37949 and Welch Foundation grant F-1607. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
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