Intestine-specific expression of Apobec-1 rescues apolipoprotein B RNA editing and alters chylomicron production in Apobec1 -/- mice.

Intestinal apolipoprotein B (apoB) mRNA undergoes C-to-U editing, mediated by the catalytic deaminase apobec-1, which results in translation of apoB48. Apobec1(-/-) mice produce only apoB100 and secrete larger chylomicron particles than those observed in wild-type (WT) mice. Here we show that transgenic rescue of intestinal apobec-1 expression (Apobec1(Int/O)) restores C-to-U RNA editing of apoB mRNA in vivo, including the canonical site at position 6666 and also at approximately 20 other newly identified downstream sites present in WT mice. The small intestine of Apobec1(Int/O) mice produces only apoB48, and the liver produces only apoB100. Serum chylomicron particles were smaller in Apobec1(Int/O) mice compared with those from Apobec1(-/-) mice, and the predominant fraction of serum apoB48 in Apobec1(Int/O) mice migrated in lipoproteins smaller than chylomicrons, even when these mice were fed a high-fat diet. Because apoB48 arises exclusively from the intestine in Apobec1(Int/O) mice and intestinal apoB48 synthesis and secretion rates were comparable to WT mice, we were able to infer the major sites of origin of serum apoB48 in WT mice. Our findings imply that less than 25% of serum apoB48 in WT mice arises from the intestine, with the majority originating from the liver.

However, several features of mammalian intestinal apoB RNA editing and the functional signifi cance of apobec-1 remain incompletely understood. Earlier studies indicated that transgenic overexpression of apobec-1 caused C-to-U hyperediting at multiple sites (including the canonical nucleotide) in hepatic apoB RNA both in vivo ( 12 ) and in hepatoma cell lines ( 13 ). These fi ndings raised questions of how C-to-U RNA editing at the canonical site is regulated physiologically and whether hyperediting might be demonstrated upon apobec-1 overexpression in nonhepatic tissues ( 14,15 ). In addition, as alluded to above, the importance of intestinal apoB48 and its contribution to serum apoB48 levels in the mouse has been diffi cult to discern, at least in part because mouse liver secretes both isoforms ( 7 ). Here we use a strategy of transgenic rescue to reveal unanticipated sites of C-to-U editing in intestinal apoB RNA and to characterize apoB-containing lipoproteins in mice expressing only apoB48 in the small intestine.

Generation of transgenic animals
The coding region of human apobec-1 was cloned into pGEM-AclI-villin-EGFP-KpnI-BGHpolyA-AclI vector (a gift from Dr. J. Turner, University of Chicago). The 711 bp coding region was inserted into the unique KpnI site downstream of EGFP motif, resulting in the expression of a N-terminal EGFP-tagged human Apobec-1. The expression of the transgene was under the control of a 9 kb villin promoter ( 16 ). This construct ( Fig. 1A ) was microinjected into fertilized eggs from C57BL/6 × CBA mice. Apobec-1 transgenic mice were then mated with C57BL/6 Apobec1 Ϫ / Ϫ mice to generate lines of Apobec-1 Int/O animals expressing Apobec-1 only in the intestine.

Northern blot analysis and semiquantitative PCR
Intestinal segments were fl ushed and scraped mucosa was fl ashfrozen in liquid nitrogen for total RNA extraction. Total RNA (20 µg) prepared in 1× MOPS, 6.7% formaldehyde, 72% formamide, and 40 g/ml ethidium bromide was subjected to denaturing formaldehyde/1.2% agarose electrophoresis and transferred to Imobilon-NY+ membrane (Millipore, Billerica, MA). Membranes were prehybridized and hybridized in ExpressHyb hybridization solution (Clontech Laboratories, Mountain View, CA) at 70 ° C when probing for apobec-1 or 76 ° C when probing with GFP. Apobec-1 and GFP probes (445 nt) generated by PCR were labeled by random priming using [ 32 P]dATP and Klenow (NEB Biolabs, Ipswich, MA). Apobec-1 probe was generated using the following primers: Fwd H/M 34: 5 ′ -CCCACTCTGAGGAGAAG-3 ′ and Rev H/M 479: 5 ′ -GGTAGTTGACGAAATTCCTCCAGCAG-3 ′ . Washes were performed at room temperature for 40 min in 2× SSC, 0.05% SDS, followed by two washes at 50 ° C in 0.1× SSC, 0.1% SDS. Membranes were exposed to PhosphorImager SI (Molecular Dynamics, Sunnyvale, CA). Integrity and loading were monitored by visualization of ribosomal subunits. For semiquantitative evaluation of human Apobec-1 RNA expression, total RNA from wildtype, Apobec-1   ( 18 ). At the end of chase, medium and cells were collected, and aliquots of lysate and medium were immunoprecipitated with rabbit anti-mouse apoB IgG. Quantitation of [ 35 S]incorporation into apoB48 was conducted using 4-15% SDS-PAGE gel separation of the immunoprecipitation reactions, which were then quantifi ed using PhosphorImager analysis (Molecular Dynamics, Sunnyvale, CA).

Lipoprotein fractionation by fast-pressure liquid chromatography
Animals were fed chow or a Western diet (Harlan Teklad #TD 88137, Madison, WI) as indicated for 10-12 weeks before study. After an overnight fast, animals were weighed and injected intravenously with Pluronic F127 ( 19 ), followed 30 min later by an intragastric bolus of 0.5 ml of a lipid mixture containing 100 µl corn oil and 400 µl 20% intralipid. Blood was collected before Pluronic F127 injection (time 0) and 4 h after lipid gavage. Serum was recovered by centrifugation at 4,000 rpm for 20 min at 4°C. Pooled serum (100 µl) was analyzed by fast-pressure liquid chromatography (FPLC) using two Superose 6 columns connected in series (GE Healthcare Life Sciences, Pittsburgh, PA). Each FPLC run yielded 56 fractions of 500 µl each. Aliquots of each individual fraction (30 µl) were resolved by 4-15% SDS-PAGE, and the distribution of apoB, apoA1, apoA4, and apoE was determined by Western blot. Cholesterol and triglyceride content in each fraction was determined enzymatically using Cholesterol E and L-Type Triglyceride M kits (Wako Chemicals, Richmond, VA).

Electron microscopy
Pooled serum (200 µl) collected 4 h after lipid gavage was layered under 600 µl 0.15 M NaCl and centrifuged at 50,000 rpm for 30 min in the MLA-130 rotor in a tabletop ultracentrifuge (Beckman Instruments). Chylomicrons were collected and submitted to negative staining electron microscopy, and then visualized using a Zeiss 902 electron microscope. At the time of sacrifi ce (4 h post-lipid gavage), 2 mm segments of the jejunum were fl ushed with PBS followed by immersion in fi xative solution containing 3% Glutaradehyde (EM grade); 1% formaldehyde (EM grade) in 0.1 M sodium cacodylate (pH 7.4); 2 mM Cacl 2 ; and 2 mM MgCl 2 . Specimens were kept at 4°C in 1.5 ml fi xative, stained in 2% aqueous low-expressor (L) animals was treated with DNase (Ambion, Foster City, CA) and used to synthesize cDNA. A 220-nt motif targeting exon 6 of Apobec-1 (supplementary Fig. I)  PCR products were resolved on a 1% agarose gel and quantitated using Kodak/Image Digital Science and Carestream Molecular Imaging System software. Apobec-1 PCR products were normalized to GAPDH. Quantitative PCR was performed using individual samples (3-4 per genotype). For each sample, reactions were performed in triplicate on an ABI Prism 7000 sequence detection system using SYBR GreenER PCR Master Mix (Invitrogen, Grand Island, NY) and primers designed by Primer Express software (Applied Biosystems). Murine Apobec-1-specifi c primers were as follows: Fwd: 5 ′ -TGTTTATTTACATAGCACGGCTTTATC-3 ′ and Rev:

ApoB RNA editing analysis by primer extension and sequencing
RNA was isolated from scraped mucosa using TRIzol (Invitrogen, Grand Island, NY). DNase-treated RNA (1 µg) was used for primer extension analysis of apoB RNA editing as previously detailed ( 17 ). Sequence analysis of apoB RNA hyperediting was conducted on a 738-nt region spanning nucleotides 6508 to 7246, amplifi ed by RT-PCR using total RNA isolated from scraped mucosa of WT, Apobec-1 Ϫ / Ϫ , and Apobec-1 Int/O mice. PCR products were purifi ed and subcloned into pPCR-Script SK(+) plasmid (Agilent Technologies/Stratagene, La Jolla, CA). Twenty individual clones were sequenced using Big Dye terminator mix. Sequences were aligned with SerialCloner 3-1 software.

Enterocyte isolation and pulse chase analysis of apoB secretion
Enterocytes were isolated using EDTA chelation from four individual mice per genotype and used for pulse-chase experiments as described ( 18 ). In brief, freshly isolated enterocytes were pulse labeled for 30 min with 250 µCi [ 35 S]-protein labeling mix (Cat# NEG072, PerkinElmer, Boston, MA) and chased for 60 min in DMEM supplemented with 10 mM methionine and 5 mM cysteine. was more in line with the semiquantitative RT-PCR data. Transgenic rescue in these lines was confi rmed by immunohistochemical localization of the fusion protein, which indicated homogeneous expression in villus enterocytes in both nuclear and cytoplasmic compartments ( Fig. 1E ). Electron micrographs of jejunal enterocytes from chowfed mice revealed comparable morphology between WT, Apobec1 Ϫ / Ϫ , and Apobec1 Int/O mice without changes in lipid droplet accumulation ( Fig. 1F ). Other parameters of intestinal lipid metabolism are detailed in Table 1 and discussed later.
ApoB C-to-U RNA editing in the intestine of Apobec-1 Ϫ / Ϫ mice Intestinal RNA was examined by primer extension assay ( 17 ) to determine the extent of C-to-U editing of endogenous murine apoB RNA at the canonical site. WT mice showed greater than 90% C-to-U editing, whereas Apobec1 Ϫ / Ϫ mice demonstrated no RNA editing, as expected ( Fig. 2A , B ). Transgenic rescue of apobec-1 in both lines of Apobec1 Int/O mice also revealed greater than 90% C-to-U editing at the canonical site, indicating that the transgene is fully functional with regard to its physiological target ( Fig. 2A, B ).
We next asked whether transgenic rescue of apobec-1 was associated with changes in cytidine deamination of other targets in apoB RNA, as prior studies in transgenic mouse and rabbit liver had indicated that overexpression of apobec-1 induced promiscuous hyperediting ( 12,20 ). We undertook Sanger sequencing of cDNA clones from a 738 nt fragment spanning nt 6508-7246, including the region from nt 6643-6851 examined in that earlier study ( 20 ). Our fi ndings demonstrate that C-to-U RNA editing is detectable in many sites 3 ′ to the canonical target at position 6666 and, importantly, that these RNA modifi cations were found in both WT and Apobec1 Int/O mice (high expressor) ( Fig. 2C ). The data show that the extent of C-to-U editing varies across the sites, with a maximum of 30% editing at 6987 and generally lower levels ( ‫ف‬ 10%) at other sites ( Fig. 2C ). The fi ndings reveal sites at which C-to-U uranyl acetate, and viewed on a Hitachi H-600 electron microscope (Hitachi High Technologies, Schaumburg, IL). Three animals per genotype were examined to obtain representative images.

Statistical comparisons
All data are shown as mean ± SE unless otherwise noted. Statistical comparisons were made using GraphPad Prism 4.0 (Graph-Pad, San Diego, CA) with one-way ANOVA for multiple group comparisons and t -testing as a posthoc test for comparing different pairs. A value of P < 0.05 was considered signifi cant.

Generation of intestine-only Apobec-1 (Apobec-1
Three founder transgenic lines were generated using the construct shown in Fig. 1A . For the purposes of this report, we focused on two lines in which human apobec-1 was expressed homogeneously in the small intestine at either a relatively high or low level (defi ned below) when compared with endogenous murine apobec-1. The apobec-1 intestinal transgenic founders were then crossed into the Apobec1 Ϫ / Ϫ line to generate lines of Apobec1 Int/O mice. Northern blot analysis revealed a strong signal only with the high-expressor line ( Fig. 1B ). The relative expression levels of transgenic apobec-1 mRNA were determined in comparison to endogenous murine apobec-1 by semiquantitative PCR targeting a conserved region within murine exon 6 (supplementary Figs. I and II). These data indicate a range of   The fi ndings with regard to the sites of hyperediting of intestinal apoB RNA contrast with those demonstrated earlier for hepatic apoB RNA in liver-specifi c apobec-1 transgenic mice ( 20 ), in which a major cluster of cytidine residues at positions 6738--6762 and another cluster at 6802-6812 were each observed to undergo C-to-U hyperediting. None of those sites were found to undergo C-to-U editing in mouse intestine in either WT or Apobec1 Int/O mice ( Fig. 2C ). These fi ndings strongly suggest that site selectivity of apoB RNA modifi cations is infl uenced in a tissue-specifi c fashion. We checked whether targeting of these additional sites was mooring sequence-dependent ( 13,20 ). When compared with the canonical mooring sequence, we identifi ed only one site (7017) with an almost perfect match with the consensus motif ( Fig. 2D ). However, editing effi ciency at this site ( ‫ف‬ 10%) was similar to other sites (6933, 6990, 7085, and 7187) with more mismatches to the mooring sequence, suggesting that the presence of this motif is not a critical determinant of site selection ( Fig. 2D ). We also examined the nearest neighbor nucleotide preference surrounding editing sites with frequency higher than 10%. The nucleotide immediately upstream of the targeted cytidine (position Ϫ 1) is an adenosine (70%) or guanosine (28%), compared with the immediate downstream nucleotide, adenosine (43%), uridine (43%), or guanosine (14%) ( Fig. 2E ). These fi ndings contrast with the nearest neighbor preferences identifi ed for liver hyperediting in which the upstream pre ference was for thymidine (70%) or adenosine (30%) ( 20 ). The fi ndings together suggest that sequence-specifi c (contextual) elements interact with tissue-specifi c factors in the specifi city of apobec-1 mediated C-to-U RNA editing of apoB.
We also examined these patterns of C-to-U RNA editing in the low-expressor line of Apobec1 Int/O mice since earlier work indicated a dose response for hyperediting in apobec-1 transgenic liver ( 21,22 ). Our fi ndings demonstrate that low-expressor Apobec1 Int/O mice exhibit reduced levels of hyperediting compared with both WT and the high-expressor Apobec1 Int/O line, with the dominant location again at the 6987 site ( Fig. 2F ).
RNA editing was found only in the Apobec1 Int/O mice (e.g., 6933, 6990, and 7187) and also sites in which C-to-U RNA editing was only found in the WT intestine (6998, 7036, and 7120). However, for the most part, there was concordance in the patterns observed between WT and Apobec1 Int/O mice. The observed pattern of C-to-U RNA editing of these additional sites does not appear to be processive (5 ′ → 3 ′ or 3 ′ → 5 ′ ) based on the fi nding that none of the sites appear linked to one another. One additional editing site (1/20 clones) was identifi ed (6639) 5 ′ to the canonical base, changing a CUC (Leu) to UUC (Phe), but all the other changes within the 738 nucleotides examined were found 3 ′ to the canonical site, which was quantitatively edited. Whether additional sites for C-to-U RNA editing exist in exon 26 upstream of nucleotide 6508 or in other 5 ′ exons remains to be determined, but we will return to this question later.   Taken together, the fi ndings reveal an unanticipated array of targets for C-to-U RNA editing in WT murine intestine that is eliminated in Apobec1 Ϫ / Ϫ mice (data not shown) and largely restored in a dose-dependent manner by transgenic rescue in Apobec1 Int/O mice. For the purposes of the functional characterization (detailed below), we used Apobec1 Int/O mice expressing high levels of the transgene.

Intestinal apoB48 production in Apobec1 Int/O mice
We examined apoB isoform expression in mice of the indicated genotypes, which revealed that apoB48 was the dominant intestinal isoform expressed in Apobec1 Int/O mice and that there were no other truncated species detectable either in serum or intestinal mucosa ( Fig. 3A , B ). We next examined apoB48 synthesis and secretion in isolated enterocytes from WT and Apobec1 Int/O mice, the fi ndings demonstrating comparable synthesis and secretion rates with no differences in the overall recovery of apoB ( Fig. 4A -D ). These fi ndings demonstrate that intestine-specifi c apobec-1 transgenic expression rescues the patterns of synthesis and secretion of intestinal apoB48 in Apobec1 Int/O mice. In addition, there was no discernable difference between WT and Apobec1 Int/O mice in terms of weight gain or lipid absorption (data not shown) or in terms of intestinal or fasting administration). Accordingly, we constructed a semiquantitative standard curve of serum apoB48 in both chow- ( Fig. 8A ) and Western diet-fed mice ( Fig. 8B ) using serial dilutions to obtain comparable apoB48 abundance under each dietary condition. The fi ndings ( Fig. 8A, B ) imply that the intestine contributes ‫ف‬ 10-25% of total serum apoB48, with the majority of apoB48 production refl ecting hepatic secretion.

DISCUSSION
The key fi ndings from this study demonstrate that transgenic expression of human apobec-1 in the intestine of Apobec1 Int/O mice rescues apoB RNA editing at the canonical site (6666), restores intestinal apoB48 production, and produces a shift in the spectrum of intestinal lipoproteins. The fi ndings also reveal an unanticipated number of additional sites of C-to-U RNA editing of intestinal apoB, including a newly identifi ed cluster of sites that were present not only in Apobec1 Int/O mice in which apobec-1 was overexpressed but also in WT animals. These features together raise important implications for our understanding of the regulation of posttranscriptional C-to-U RNA editing and the functional importance of apoB RNA editing in the assembly and secretion of intestinal lipoproteins. Each of these features merits additional discussion.
Considerable effort has been devoted to understanding the cis -acting elements and trans -acting factors that regulate C-to-U RNA editing of apoB ( 12,13,20,23 ). Historically, this work focused predominantly on C-to-U editing serum cholesterol or triglyceride concentrations either on a chow or Western diet ( Table 1 ). These fi ndings would be predicted based on the predominant pattern of intestinal apoB48 production in WT mice.

Serum apoB isoform and lipoprotein distribution in Apobec1 Int/O mice
We next turned our attention to the distribution pattern of apoB isoforms in Apobec1 Int/O mice, as these mice produce apoB48 exclusively in the intestine and apoB100 exclusively in the liver. Following Pluronic F127 administration, we found that the net (representing both hepatic plus intestinal) secretion rate of triglyceride-rich lipoproteins was comparable but with reduced abundance of apoB48 in Apobec1 Int/O mice compared with WT 4 h following a lipid bolus ( Fig. 5A , B; see also Fig. 3B ). The distribution of isoforms across the lipoprotein profi le revealed a subtle change in apoB48 distribution by genotype. ApoB48 fractionated into chylomicron/VLDL-sized particles in both WT and Apobec-1 Int/O mice ( Fig. 5C, E ), but apoB48 distributed into a more homogeneous population of LDL particles in Apobec-1 Int/O mice ( Fig. 5E , fractions 24-28) compared with WT mice, where apoB48 appeared in broad population of LDL-sized particles ( Fig. 5C , fractions [18][19][20][21][22][23][24][25][26][27][28][29]. Triglyceride distribution was indistinguishable between the genotypes, almost exclusively within chylomicron and VLDL fractions, as expected ( Fig. 5D, F ).
We next evaluated the size distribution of chylomicron and VLDL particles from the indicated genotypes using negative-stain electron microscopy, which revealed a shift to a smaller population of particles in Apobec1 Int/O mice ( Fig. 6 ), again suggesting that intestinal lipoprotein production is altered upon rescue of intestinal apoB48 production.
The fi ndings to this point suggest that there is a shift in the profi le of intestinal lipoproteins in Apobec1 Int/O mice. We extended this characterization to mice fed a high-fat Western diet (see Table 1 for lipid data) in which the FPLC profi le again revealed that only a fraction of apoB48 from Apobec1 Int/O mice distributed into chylomicron/VLDL-sized particles ( Fig. 7A -C ). As noted above in chow-fed mice, triglycerides distributed virtually exclusively in chylomicron and VLDL fractions. We also examined the distribution of apoE and apoA1, which revealed comparable distribution in chylomicron and VLDL fractions of both genotypes ( Fig. 7D ). By contrast, apoE and apoA1 were found in the small LDL/large HDL-sized range in Apobec1 Int/O mice ( Fig. 7D , bracketed fractions), suggesting again a distinctive pattern of particle distribution in association with intestinal apoB48 in these mice.
Finally, because apoB48 arises exclusively from the intestine of Apobec1 Int/O mice and because intestinal apoB48 synthesis and secretion rates (as inferred from our in-vitro studies in isolated enterocytes; see Fig. 4 ) were comparable between the genotypes, we reasoned that it would be feasible to infer the contribution of intestinal apoB48 production to serum apoB48 levels in WT mice under conditions where clearance of intestinal and hepatic apoB48 particles was eliminated (i.e., following Pluronic F127  of synthetic apoB RNA templates fl anking the canonical site and indicated both nearest neighbor preferences ( 23,24 ) and also distinct structural context requirements ( 25,26 ). These RNA elements, together with regulated abundance of apobec-1 and its auxiliary components, including ACF, were viewed as suffi cient and necessary to constrain C-to-U editing of apoB to a physiological site at position 6666 ( 6 ). However, the fi nding that forced overexpression of apobec-1 induced hyperediting of apoB RNA at multiple sites suggested that these constraints could be overcome ( 13,20 ). The current fi ndings illustrate several important contrasts from those earlier studies. First, almost none of the sites identifi ed as targets of hyperediting in apobec-1 transgenic mouse and in rabbit liver apoB RNA by Yamanaka et al. ( 20 ) were found to be edited in intestinal apoB RNA in Apobec1 Int/O mice. This includes the 6802 site, which was identifi ed earlier in human intestinal cDNA as an example of noncanonical C-to-U RNA editing ( 27 ). These fi ndings demonstrate that target specifi city for C-to-U RNA editing of apoB is regulated in a tissue-specifi c manner and that distinctive factors constrain and regulate the extent and effi ciency of hepatic versus intestinal apoB RNA editing, particularly under conditions where apobec-1 expression may be altered. The second important feature is that noncanonical sites for C-to-U editing, in particular the cluster of targets between 6987 and 7187, were found in both WT and Apobec1 Int/O mice albeit at lower effi ciency (up to 30%) compared with the canonical site. These fi ndings imply that C-to-U RNA editing of murine intestinal apoB is not confi ned to a single site, even under circumstances where apobec-1 is expressed at physiological levels. These fi ndings contrast with earlier observations in murine liver, where none of the cDNA clones spanning nt 6643-6851 sequenced from endogenous (murine) or transgenic human apoB were edited (with the exception of 6806) ( 20 ). It will be of interest to extend those fi ndings and include the 3 ′ cluster of C-to-U editing sites identifi ed here in intestinal apoB cDNA. Those studies are currently in progress and will be reported elsewhere. The predominant overlap in hyperediting site selection and effi ciency noted in WT and the high-expressing Apobec1 Int/O mice suggest that simply overexpressing human (versus murine) apobec-1 in murine intestine is unlikely to account for the fi ndings. The observation that hyperediting of apoB RNA involved fewer noncanonical sites in the low-expressor line of Apobec1 Int/O mice (again, largely overlapping sites observed in WT mice) further supports the conclusion that human and murine apobec-1 exhibit similar functional characteristics with regard to murine intestinal apoB RNA editing in vivo. These conclusions are broadly consistent with the fi ndings from rabbit apobec-1 transgenic overexpression in murine liver and from in-vitro studies in human and rat hepatoma cells ( 20,24 ). However, recent fi ndings using more sensitive amplifi cation methods to detect C-to-U RNA editing events have demonstrated that adenoviral expression of rat and human apobec-1 in hepatoma cell lines exhibits different specifi city for introducing hypermutations, suggesting that tissue-specifi c cofactor interactions may be an important consideration in understanding how site selection is regulated ( 28 ).
It is also worth pointing out that virtually all the sites of C-to-U RNA editing were 3 ′ of the canonical site and that the additional RNA editing events described occur in the 3 ′ untranslated region (UTR) of the apoB transcript. Recent fi ndings using deep sequencing of intestinal RNA (RNA seq) from WT mice found 32 new (i.e., non-apoB) targets of C-to-U editing, all of which were in the 3 ′ UTR and all of which were eliminated in the intestine of Apobec1 Ϫ / Ϫ mice ( 29 ). These fi ndings, taken together . One microliter of diluted serum was resolved by 4-15% SDS-PAGE and probed using anti-apoB antibody. ApoB48 band intensity was quantitated using Kodak/Image Digital Science and the Carestream Molecular Imaging System software. Band intensities from WT apoB48 were used to create a standard curve. ApoB48 band intensity within the WT standard curve was used to evaluate the relative contribution of intestine to apoB48 production. As an example, in (A), the intensity of the band from Apobec-1 Int/O serum diluted 1:16 represents 25% of the band intensity from WT serum of the same dilution.
with the current results, indicate that there is a wider range of C-to-U editing targets than previously thought and that these targets reside within the 3 ′ UTR, raising questions regarding the functional impact of these modifi cations. It will be important to undertake a comprehensive analysis of the entire apoB transcript from mice of the three genotypes examined in the current study to determine whether there are additional sites of C-to-U editing beyond those identifi ed in the region of 6508-7246. As alluded to above, this analysis will extend to regions both 5 ′ and 3 ′ of the regions examined in the current report, and those studies are currently in progress. However, RNA seq studies reported earlier indicated only a low level (up to 10%) of hyperediting of cytidine residues in apoB RNA, downstream and in close proximity to the canonical site (6676 and 6708) ( 29 ). It is important to emphasize that Western blots of intestinal mucosal extracts and serum from Apobec1 Int/O mice each indicated only apoB48 and no other truncated apoB species, suggesting that there are no new functional translational termination codons created through alternative C-to-U RNA editing. That being said, it is possible that these additional RNA editing events within the 3 ′ UTR of apoB might infl uence other aspects of apoB mRNA biology, including transport and translational effi ciency. Those possibilities await formal examination.
The current studies demonstrate that intestinal apoB48 synthesis and secretion are restored in Apobec1 Int/O mice and reveal no obvious impact on the effi ciency of lipid absorption. The fi ndings indicate a subtle shift in apoB48 distribution that includes a population of smaller chylomicron particles (identifi ed by electron microscopy) whose signifi cance remains to be elucidated. In addition, the fi ndings demonstrate that the distribution of apoB48 in Apobec1 Int/O mice also includes LDL-and HDL-sized fractions. This observation raises the question of the functional relevance of apoB48 within these fractions. It is worth noting that earlier studies in apoB48-only versus apoB100-only mice demonstrated that cholesterol distributed into predominantly HDL-sized particles whereas TG distributed predominantly into chylomicron/VLDL-sized particles ( 30 ). However, those studies left open the relative contribution of intestinal versus hepatic apoB48 in the apoB48-only mice. The current fi ndings demonstrate that, following a lipid bolus, virtually all the triglyceride in serum is transported in the apoB48-containing fractions of chylomicron/VLDL size in both WT and Apobec1 Int/O mice. On the other hand, a large fraction of the apoB48 in Apobec1 Int/O mice cofractionates with smaller particles, raising the possibility that these apoB48-containing particles in the LDL and HDL range are underlipidated, precursor lipoprotein particles. This possibility will require further experimental validation but is broadly consistent with the two-step hypothesis for triglyceride-rich lipoprotein assembly and secretion as inferred from studies in the liver ( 31 ). The lipid cargo of these smaller, apoB48-containing intestinal lipoproteins remains to be defi ned more completely but our fi ndings ( Figs. 5E and 7C ) indicate that they contain cholesterol. The possibility that intestinal lipid transport utilizes different secretory pathways (i.e., chylomicron and HDL) is consistent with other work examining intestinal vitamin E ( 32 ) and cholesterol secretion ( 33 ).
The strategy for generating Apobec1 Int/O mice also provided the opportunity to examine the contribution of intestinal apoB48 production to the overall serum apoB48 pool in WT mice. We used the assumption that, because apoB48 synthesis and secretion rates were similar, as inferred from studies in isolated enterocytes, the abundance of serum apoB48 in the respective genotypes would refl ect intestinal secretion under circumstances in which apoB uptake was eliminated. The fi ndings suggest that under conditions of either chow or high-fat Western diet feeding, the intestinal contribution of apoB48 in WT mice is only 10-25% of the total. In other words, under both dietary conditions, the majority of apoB48 in WT mice originates from the liver. Following intake of a high-fat Western diet, the contribution of intestinal apoB48 was lower than in chow-fed mice, but these fi ndings should be interpreted with caution as hepatic apoB48 synthesis and secretion rates were not formally analyzed in these experiments. Nevertheless, the results suggest that the intestine accommodates chylomicron assembly and triglyceride mobilization through apoB48 production and secretion of particles in the size range of chylomicrons but in addition secretes a range of smaller particles containing apoB48 whose lipid transport function and metabolic implications are yet to be fully understood.
In summary, the fi ndings from this study illustrate an unanticipated range of targets of C-to-U apoB RNA editing, fi ndings that extend discussion regarding the diversity of DNA versus RNA differences (34)(35)(36)(37). Further questions, both in relation to C-to-U RNA editing as a biological process and in relation to apoB48 assembly and secretion as a functional pathway for intestinal lipid export, are the focus of ongoing investigation.