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Keratin 8 overexpression promotes mouse Mallory body formation
Correspondence to Bishr Omary: mbishr{at}stanford.edu
Abstract
Keratins 8 and 18 (K8/18) are major constituents of Mallory bodies (MBs), which are hepatocyte cytoplasmic inclusions seen in several liver diseases. K18-null but not K8-null or heterozygous mice form MBs, which indicates that K8 is important for MB formation. Early stages in MB genesis include K8/18 hyperphosphorylation and overexpression. We used transgenic mice that overexpress K8, K18, or K8/18 to test the importance of K8 and/or K18 in MB formation. MBs were induced by feeding 3,5-diethoxycarbonyl-1,4-dihydrocollidine (DDC). Livers of young K8 or K8/K18 overexpressors had no histological abnormalities despite increased keratin protein and phosphorylation. In aging mice, only K8-overexpressing livers spontaneously developed small "pre-MB" aggregates. Only K8-overexpressing young mice are highly susceptible to MB formation after short-term DDC feeding. Thus, the K8 to K18 ratio, rather than K8/18 overexpression by itself, plays an essential role in MB formation. K8 overexpression is sufficient to form pre-MB and primes animals to accumulate MBs upon DDC challenge, which may help explain MB formation in human liver diseases.
Abbreviations used in this paper: Ab, antibody; ALT, alanine aminotransferase; DDC, 3,5-diethoxycarbonyl-1,4-dihydrocollidine; IF, intermediate filament; MB, Mallory body; WT, wild type.
Introduction
Intermediate filaments (IFs) are a large family of cytoplasmic and nuclear proteins that are involved in a broad range of diseases that reflect their cell and tissue-specific expression (Herrmann et al., 2003; Coulombe and Wong, 2004; Omary et al., 2004). The nuclear IFs include lamins, whereas examples of cytoplasmic IFs include desmin and neurofilaments that are preferentially expressed in muscle and neuronal cells, respectively. In epithelial cells, cytoplasmic IFs consist of types I and II keratins that are found as obligate noncovalent heteropolymers and are expressed in an epithelial cell–specific manner (Coulombe and Omary, 2002). Type I and II keratins stabilize each other via formation of a coil–coil 
helix and are found in cells in a 1:1 type I/II stoichiometric ratio. In digestive organ epithelia, the major IFs are keratin polypeptides 8 and 18 (K8/18), with variable levels of K7, 19, and 20 depending on the tissue/cell type (Ku et al., 1999). Adult hepatocytes are unique in that they express K8/18 exclusively (Omary et al., 2002). The absence of either K8 or K18 results in the rapid degradation of most of the remaining keratin partner by ubiquitinylation in order to maintain the 1:1 type I/II keratin protein ratio (Kulesh et al., 1989; Ku and Omary, 2000).
An important function of K8/18 is to protect hepatocytes from mechanical and nonmechanical stresses, as demonstrated using several transgenic animal models (Omary et al., 2002; Magin et al., 2004; Zatloukal et al., 2004). For example, K8-null or K18 mutant–expressing mice are highly susceptible to liver injury, which led to the identification of K8 and K18 variants in patients with end-stage liver disease (Omary et al., 2004; Ku et al., 2005). K8/18-related liver disease likely occurs by a multi-hit process that includes the keratin mutation and other insults such as viral and toxin-related injuries (Omary et al., 2002; Ku et al., 2005). K8 and K18 are also the major components of Mallory bodies (MBs) and are essential for MB formation (Denk et al., 2000). MBs are typically noted as hyaline, irregular-shaped cytoplasmic aggregates or deposits found particularly but not exclusively in hepatocytes of patients with alcoholic and nonalcoholic steatohepatitis (Denk et al., 2000). Similar cytoplasmic deposits that contain other IFs are seen in other diseases, including astrocyte Rosenthal fibers (glial fibrillary acidic protein deposits) of Alexander disease and neurofilament deposits in several neurodegenerative diseases (Cairns et al., 2004; Omary et al., 2004; Cookson, 2005). These aggregates are hallmarks of several diseases, but the mechanism of their formation is poorly understood, albeit MBs are among the most studied as a result of mouse models that include feeding a diet containing griseofulvin or 3,5-diethoxycarbonyl-1,4-dihydrocollidine (DDC; Denk et al., 2000).
The accumulation of MBs is a multistep process that includes liver injury–mediated K8/18 hyperphosphorylation and K8/18 mRNA and protein overexpression (Yuan et al., 1996; Cadrin et al., 2000; Denk et al., 2000; Stumptner et al., 2000; Omary et al., 2002). Keratin induction is asymmetric, particularly at the protein level. For example, K8 protein increases nearly 5- and then 3-fold, whereas K18 increases nearly 2- and then 1.5-fold after 1 wk and 2.5 mo of DDC feeding, respectively (Denk et al., 2000). The increases in K8/18 mRNA are somewhat more prominent (K8, nearly sixfold; K18, nearly fivefold after 1 wk of DDC feeding; similar levels were seen after 2.5 mo of feeding; Denk et al., 2000) and are likely mediated by an increase in mRNA stability (Cadrin et al., 2000). Such differences in keratin induction are physiologically relevant because the relative K8 versus K18 levels appear to be important for MB formation. For example, aged K18-null mice (K8 > K18) spontaneously develop abnormal hepatocytes with K8-positive MB-like aggregates (Magin et al., 1998). In contrast, K8-null or heterozygous (+/–) mice (K18 > K8) do not form MBs even after intoxication with DDC (Zatloukal et al., 2000). However, differences between in vivo and cell culture models occur in that transfected K18 is more prone to aggregate than transfected K8 (Nakamichi et al., 2002). Although these studies suggest that keratins are important for MB development, the relationship between single or dual K8 and K18 overexpression and MB formation under basal and stimulated conditions remains unclear. We addressed this issue using transgenic mice that overexpress human (h) K18 (Abe and Oshima, 1990) or mouse (m) K8 or mK8/hK18. A previous study described transgenic mice that overexpressed hK8 and developed progressive chronic pancreatitis, but, although detailed analysis was not performed, no liver abnormalities were described (Casanova et al., 1999).
Results and discussion
Keratin mRNA and protein expression were analyzed in four transgenic mouse lines: single (K8 or K18) or double overexpressors (K8/18) and control wild-type (WT) nonoverexpressors. These lines were generated by mating mK8 overexpressors (EA5 +/–) together or with hK18 overexpressors (TG2 +/+; Fig. S1, available at http://www.jcb.org/cgi/content/full/jcb.200507093/DC1). Analysis of keratin transcription by real-time PCR demonstrated a 3.2-fold increase of mK8 RNA in the K8 overexpressors and a similar increase (2.5-fold) in mice that overexpressed K8/18 as compared with WT mice (Fig. 1 A). K8 overexpression had a slightly more prominent effect on K18 mRNA induction (1.8 ± 0.2) as compared with the effect of K18 overexpression on K8 (1.3 ± 0.3). As expected, hK18 mRNA was detected in the K18 and K8/18 overexpressors (Fig. 1 A). Keratin protein overexpression paralleled the mRNA changes (Fig. 1 B). For example, mK8 protein increased 
2.5-fold in the K8 and K8/18 overexpressors (see Protein analysis). K8 overexpression has a more profound impact on K18 protein induction as compared with K18 overexpression on K8 protein induction, and K8 + K18 protein levels are highest in the K8/18 double and K8 overexpressors (Fig. 1 B). Therefore, of the K8, 18, or 8/18 lines, the normal 1:1 K8 to K18 liver protein ratio is best approximated in the K8/18 overexpressors while yielding a nearly 2.5-fold increase in overall keratin protein.
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Given that MBs form spontaneously in old but not in young K18-null mice (Magin et al., 1998), we asked whether keratin deposits form in old mouse livers isolated from WT, K8, K18, and K8/18 mice. Notably, livers from 2-yr-old K8 mice develop keratin aggregates of varied sizes, whereas livers of similarly aged WT, K18, or K8/18 mice do not (Fig. 2). The keratin aggregates consist of small dots located primarily near the cell periphery and of larger, MB-like cytoplasmic aggregates, which also stained positive for K18 pS33 (Fig. 2, C and D) even though clear MB formation was not seen by histochemical staining (not depicted). The larger keratin-containing aggregates uniformly included ubiquitin, whereas the smaller dots did not (Fig. 2, C and D; insets). Some hepatocytes from K8/18 mice had brighter keratin staining, but keratin aggregates were rarely found (Fig. 2, G and H). The K8 aggregates excluded 
-tubulin and, thus, were not related to centrosomes nor to apoptosis, as they did not stain with an Ab specific to an apoptotic K18 fragment, and most did not colocalize with autophagosomes (Fig. S2, available at http://www.jcb.org/cgi/content/full/jcb.200507093/DC1). Altogether, we hypothesize that the keratin aggregates noted in the K8-overexpressing old mice represent pre-MBs as defined by the formation of K8/18-ubiquitin aggregates that are not easily seen by histochemical staining.
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K18 or K18 > K8 (Fig. 5 B). The model predicts that human diseases that associate with MB formation, such as alcohol-related liver injury and nonalcoholic steatohepatitis (Fleming and McGee, 1984; Neuschwander-Tetri and Caldwell, 2003; Zatloukal et al., 2004), are more likely to result in a K8 > K18 protein imbalance (K8 > K18). This model may extend to other heteropolymeric IFs, such as neurofilament-containing inclusions (Cairns et al., 2004; Strong et al., 2004), although it is not known whether the stoichiometry of specific neurofilament protein (or inclusion-associated internexin) induction is critical, as is the case for K8/18.
Materials and methods
Transgenic mice
Transgenic mice that overexpress human WT K18 (called TG2) were previously described and extensively used (Abe and Oshima, 1990; Ku et al., 2003; Zhou et al., 2005). For mouse K8 overexpression, a HindDIII 16-kb fragment of the Balb/c mouse K8 gene (EndoA1; Vasseur et al., 1985) was injected into zygotes of FVB/n mice. Four independent founder lines (EA2–EA5) were initially selected, from which the EA5 line was propagated further. Double K8/18-overexpressing mice were generated by mating homozygous (+/+) TG2 and EA5 mice. The presence of transgenes was verified by PCR screening of genomic DNA isolated from mouse tails using specific primers (Table S1, available at http://www.jcb.org/cgi/content/full/jcb.200507093/DC1). The primers that were selected to distinguish between BALB/c and endogenous FVB/n utilize an intronic K8 polymorphism that is found in the FVB/n background.
Animal feeding and tissue experiments
Mice were killed by CO2 inhalation, and blood was collected by intracardiac puncture. Livers were rapidly removed and divided into slices or pieces that were immediately fixed in 10% formalin (histology), were embedded in optimal cutting temperature (Miles; immunofluorescence staining), or were snap frozen in liquid N2 (protein/RNA analysis). Fixed tissues were sectioned and stained using hematoxylin and eosin (Histo-tec Laboratory). Immunofluorescence staining was performed as described previously (Ku et al., 2004) using Texas red–conjugated anti–rabbit (Invitrogen) and FITC-conjugated anti–mouse (Biosource International) secondary Abs. Images were taken using 100x/NA 1.40 or 60x/NA 1.40 oil lenses (Nikon) and a microscope (TE300; Nikon) combined with a confocal microscope (MRC1024ES; Bio-Rad Laboratories) and the Lasersharp software (Carl Zeiss MicroImaging, Inc.). Images were compiled using Adobe Illustrator or Adobe Photoshop software. Conventional and immune electron microscopy were performed as described previously (Toivola et al., 2000), and samples were viewed and photographed using an electron microscope (CM-12; Philips). Serologic tests included aspartate aminotransferase and ALT, alkaline phosphatase, total bilirubin, creatinine, and amylase. For MB induction, sex-matched mice (3–4-mo old; three males and two females for each genotype) were fed a powdered Formulab Diet 5008 (Deans Animal Feeds) containing 0.1% DDC (Sigma-Aldrich) for 6 wk (instead of the typical 3-mo feeding; Zatloukal et al., 2000). The diet was replenished every 2 d. Statistical analysis for ALT was performed using Dunnett's method and for MB quantification using the t test. For MB quantification, 10 randomly selected high power fields were used per genotype, and the number of hepatocytes with MBs were counted and presented as means ± SD.
Protein analysis
Total protein tissue lysates were prepared by homogenization in 2% SDS-containing sample buffer and analyzed by SDS-PAGE followed by transfer to membranes for immunoblotting and visualization by enhanced chemiluminescence. The Abs used included (Ku et al., 2004) the following: rabbit Ab 8592 (anti-m/hK8/K18) and Ab 8250 (anti-K18 pS33); rat Troma I (anti-mK8) and Troma II (anti-mK18); mouse Ab L2A1 (anti-hK18) and Ab LJ4 (anti-mK8 pS79); mouse antiactin and anti-hsp60 (NeoMarkers); mouse anti–-tubulin (Sigma-Aldrich); mouse Ab M30 (anti-K18 apoptotic fragment; Roche); anti–microtubule-associated protein light chain 3 (a gift from R. Kopito, Stanford University, Palo Alto, CA); and mouse anti-p62 and antiubiquitin (Santa Cruz Biotechnology, Inc.). Keratin protein induction was quantified by densitometric scanning of blots containing serial dilutions of whole liver homogenates from the transgenic lines (analyzed on the same gel).
Real-time RT-PCR
Total RNA was isolated using an RNeasy Midi Kit (QIAGEN). The RNA was translated into cDNA using oligo-dT primers and Superscript II reverse transcriptase (Invitrogen). Quantitative real-time PCR was performed with a Sequence Detection System (ABI Prism 7900; PE Biosystems) and specific primers (Table S1). Samples were analyzed in quadruplicates, and at least three individual mice were tested for each genotype. L7 ribosomal protein was used as an internal control, and keratin and actin cDNA levels were normalized so that L7 expression was near equal in all tested mice. After confirming that the amplification efficiency was similar for all genes, transcript levels relative to L7 were determined and reported as means ± SD.
Online supplemental material
Fig. S1 shows breeding and screening of WT, K8, K18, and K8/18 lines. Fig. S2 shows characterization of keratin aggregates in aging K8 mice. Table S1 shows sequences of PCR primers used for K8 and K18 transgene screening and sequences of primers used for real-time PCR.
Acknowledgments
We are grateful to Ron Kopito for the antibody gift, Nafisa Ghori for help with electron microscopy, Karin Zeh and Jacqueline Avis for initial work on the K8 mice, Evelyn Resurreccion for assistance with tissue sectioning and immunofluorescence staining, and Kris Morrow for assistance with figure preparation.
This work was supported by the National Institutes of Health (NIH) grant DK52951 and the Department of Veterans Affairs Merit Award (M.B. Omary) as well as the NIH Digestive Disease Center grant DK56339. P. Strnad is supported by a long-term European Molecular Biology Organization postdoctoral fellowship.
Submitted: 19 July 2005
Accepted: 11 November 2005
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