A disease- and phosphorylation-related nonmechanical function for keratin 8

doi:10.1083/jcb.200602146

Published 3 July 2006. doi:10.1083/jcb.200602146
The Rockefeller University Press, 0021-9525 $8.00
JCB, Volume 174, Number 1, 115-125

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A disease- and phosphorylation-related nonmechanical function for keratin 8

Nam-On Ku and M. Bishr Omary

Department of Medicine, Palo Alto VA Medical Center and Stanford University School of Medicine, Palo Alto, CA 94304

Correspondence to Nam-On Ku: namonku{at}stanford.edu

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Keratin 8 (K8) variants predispose to human liver injury viapoorly understood mechanisms. We generated transgenic mice thatoverexpress the human disease-associated K8 Gly61-to-Cys (G61C)variant and showed that G61C predisposes to liver injury andapoptosis and dramatically inhibits K8 phosphorylation at serine73 (S73) via stress-activated kinases. This led us to generatemice that overexpress K8 S73-to-Ala (S73A), which mimicked thesusceptibility of K8 G61C mice to injury, thereby providinga molecular link between K8 phosphorylation and disease-associatedmutation. Upon apoptotic stimulation, G61C and S73A hepatocyteshave persistent and increased nonkeratin proapoptotic substratephosphorylation by stress-activated kinases, compared with wild-typehepatocytes, in association with an inability to phosphorylateK8 S73. Our findings provide the first direct link between patient-relatedhuman keratin variants and liver disease predisposition. Thehighly abundant cytoskeletal protein K8, and possibly otherkeratins with the conserved S73-containing phosphoepitope, canprotect tissue from injury by serving as a phosphate "sponge"for stress-activated kinases and thereby provide a novel nonmechanicalfunction for intermediate filament proteins.

Abbreviations used in this paper: Ab, antibody; CREB, cAMP responseelement binding protein; EBS, epidermolysis bullosa simplex;HSE, high salt extraction; IF, intermediate filament; K, keratin;MLR, microcystin-LR; SAPK, stress-activated protein kinase;WT, wild type.

Introduction

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Keratins are intermediate filament (IF) proteins that are preferentiallyexpressed in epithelial cells and epidermal appendages (Fuchs and Weber, 1994;Coulombe and Omary, 2002). In epithelial cells, the prominentIFs include keratins 1–20 (K1–K20), which are furtherclassified into type I (K9–K20) and II (K1–K8) keratins,which form obligate, noncovalent type I/II keratin heteropolymers(Moll et al., 1982; Herrmann and Aebi, 2004). Unique keratincomplements serve as cell-specific markers that distinguishdifferent epithelial cell types. For example, basal epidermalkeratinocytes preferentially express K5/K14, and suprabasalkeratinocytes in the upper layer of the skin express K1/K10,whereas K8/K18 are the IF proteins of adult hepatocytes (Moll et al., 1982;Coulombe and Omary, 2002). K8/K18 is also the prototype keratinpair of simple-type epithelia and, as such, is broadly expressedin epithelial components of glandular tissues, including thepancreas and intestine, with variable levels of K19, K20, andK7, depending on the cell type (Ku et al., 1999). All IF proteins,including keratins, contain a central and conserved coiled coil–forming ${alpha}$ -helical "rod" domain that is flanked by relatively nonconservednon– ${alpha}$ -helical NH₂-terminal "head" and COOH-terminal "tail"domains (Fuchs and Weber, 1994; Herrmann and Aebi, 2004). Theflanking head and tail domains are the more exposed portionsof IF proteins, which explains why all IF phosphorylation sitesreside in these domains (Omary et al., 1998). Several in vivoK8/K18 phosphorylation sites have been identified that includeK8 Ser23/Ser73/Ser431 and K18 Ser33/Ser52 (Omary et al., 1998).K8/K18 hyperphosphorylation correlates with disease progressionin patients with chronic liver disease (Toivola et al., 2004;Zatloukal et al., 2004) and plays an essential role in regulatingkeratin filament organization, association with binding partnerssuch as 14-3-3 proteins, and turnover (Coulombe and Omary, 2002).

Keratin mutations are associated with several skin, oral, esophageal,ocular, hair, and liver diseases that reflect the tissue-specificexpression of the particular keratin (Fuchs and Cleveland, 1998;Omary et al., 2004). The resulting disease-related tissue defectsare manifestations of the clearly defined function of keratinsthat allows cells to cope with mechanical stresses. This keratin-relatedcytoprotective effect is most evident in the keratinocyte fragilityphenotype of human epidermolysis bullosa simplex (EBS), whichis caused by K5/K14 mutations, and is evident in the phenotypesof several animal models that lack or express mutant keratins(Fuchs and Cleveland, 1998; Magin et al., 2004; Omary et al., 2004).Emerging evidence also indicates that keratins protect cellsfrom nonmechanical injury via mechanisms that include keratinregulation of cell signaling cascades, regulation of susceptibilityto apoptosis, and modulation of protein targeting to subcellularcompartments (Coulombe and Omary, 2002; Toivola et al., 2005).For example, livers of K8- or K18-null mice or mice that expressK18 Arg89-to-Cys (an EBS-like mutation) manifest a remarkablepredisposition to injury and apoptosis (Ku et al., 1996, 2003;Loranger et al., 1997; Caulin et al., 2000; Gilbert et al., 2001).K18 R89C and K14 R125 residues and their surrounding amino acidsare highly conserved, and K14 R125 mutations cause the severestform of EBS and are the most common in keratin-related skindiseases (Fuchs and Cleveland, 1998; Porter and Lane, 2003).

Most human keratin-associated diseases are caused by autosomal-dominantkeratin missense mutations with near complete penetrance, andmost of these mutations are located at highly conserved regionsat the ends of the rod domain (Porter and Lane, 2003; Omary et al., 2004).Exceptions include mutations in K8/K18, which pose a risk forthe subsequent development of cirrhosis and liver disease progression(Ku et al., 1997, 2001, 2005; Strnad et al., 2006a,b), and mayalso be associated with inflammatory bowel disease (Owens et al., 2004).All known human K8/K18 mutations do not involve the highly conservedends of the rod domain. For example, the EBS-like K18 Arg89-to-Cysmutation, which causes hepatocyte fragility and predisposesto hepatocyte injury and apoptosis in mice (Ku et al., 1995,1996, 2003), has not been found in humans, and it is hypothesizedthat such mutations are embryolethal (Omary et al., 2002; Porter and Lane, 2003).The prevalence odds ratio for the association of K8/K18 mutationswith human cirrhosis is 3.8 (95% confidence interval of 2.1–7.1),and the association with liver disease is highly significantwhen comparing a large American cohort of liver disease patientswho underwent liver transplantation with a control group (P< 0.0001; Ku et al., 2005). In addition, a study using alarge German patient cohort with chronic hepatitis C showeda significant association of exonic K8 variants with increasedfibrosis (Strnad et al., 2006a). However, direct evidence forthe predisposition to liver injury via any natural human K8/K18mutation has not been described.

To address the in vivo significance of human liver disease–associatedkeratin mutations, we generated transgenic mice that overexpresswild-type (WT) or Gly61-to-Cys (G61C) human K8 (hK8) and comparedtheir susceptibility to stress-induced liver injury. We targetedK8 G61 for the following reasons: (a) K8 G61 is highly conservedamong type II keratins (Fig. 1 A ), (b) K8 G61C is the secondmost prevalent among K8/K18 variants that are associated withcirrhosis and fibrosis progression (Ku et al., 2005; Strnad et al., 2006a),and (c) in transfected cells, G61C interferes with keratin filamentreorganization and cross-links hK8 under oxidative conditions(Ku et al., 2001, 2005). The G61C mice unmasked an importantrelationship between K8 G61C mutation and K8 S73 phosphorylationby stress-activated protein kinases (SAPKs). This relationshipwas further explored by generating transgenic mice that overexpressK8 S73A.

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Figure 1. hK8 G61C mice have increased susceptibility to liver injury. (A) Alignment of the hK8 sequence that is proximal to G61 (shaded residue) with other type II keratins. m, mouse; r, rat; and f, frog. Single letter abbreviations are used for amino acids, and bold dots indicate amino acids that are identical to hK8. (B) Livers were isolated from nontransgenic (lane 1) or transgenic mice that overexpress hK8 WT (lanes 2 and 3) or G61C (lanes 4 and 5). Two independent transgenic lines per genotype were used (i.e., each lane from 2 to 5 represents one mouse per transgenic line). Livers were homogenized, followed by HSE to purify the total keratin pool, or were solubilized in 2% SDS-containing sample buffer to obtain total lysates (Ku et al., 2004). Isolates were separated by SDS-PAGE, and then visualized by Coomassie staining (HSE preparations) or by immunoblotting (total liver homogenates) with Abs to m/hK8, hK8, and mK18. Cross-linked K8 is detected only in livers from K8 G61C mice, and disappears if samples are analyzed under reducing conditions (not depicted). (C and D) The following three mouse genotypes were used: nontransgenic FVB/n, transgenic hK8 WT, or G61C mutant mice (16–32 age- and sex-matched mice per genotype). Each analyzed genotype consisted of nearly equal portions of the two generated independent lines (WT¹ and WT²; G61C¹ and G61C²). After Fas (C) or MLR (D) injection, mice were assessed hourly for 12 h, and then every 10 h for 3 d. The analyses show survival curves for each administered agent. (E) Summary of the mouse lethality data shown in C and D. No significant difference in mortality was observed when comparing FVB/n with hK8 WT mice, whereas mortality was markedly increased in hK8 G61C mice as compared with the combined FVB/n + hK8 WT mice.

	Results

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K8 G61C predisposes to stress-induced liver injury in transgenic mice
Transgene expression of the WT and G61C K8 mice was confirmedby blotting total liver homogenates with antibodies (Abs) specificto hK8, and by Coomassie staining of a cytoskeletal high saltextract (HSE) that shows the total liver keratin compositionand distinguishes endogenous from exogenous keratins (Fig. 1 B).Importantly, protein levels of the endogenous mouse WT K8 andhuman G61C transgene product are similar, which mimics whatis seen in human liver disease patients with heterozygous K8G61C expression. Cross-linked hK8 is found only in G61C, butnot WT, livers (Fig. 1 B) because of the absence of Cys in WThK8. Both WT and G61C mice were viable, fertile, and had noobvious phenotype under basal conditions. Previously describedtransgenic mice that overexpress high levels of WT K8, usingthe same WT hK8 we used, also do not have liver abnormalitiesunder basal conditions, but develop pancreatic insufficiencythat is possibly related to the WT hK8 expression level (Casanova et al., 1999).The K8 WT and G61C mice described herein do not have abnormalhistology in their pancreata under basal conditions (unpublisheddata).

We tested the consequence of G61C on susceptibility to liverinjury using the Fas (which causes hepatocyte apoptosis; Ku et al., 2003)or microcystin-LR (MLR; which causes hemorrhagic hepatitis;Ku et al., 1998) injury models. Fas or MLR administration causessignificant lethality (Fig. 1, C and D), and the G61C mice weremarkedly more susceptible to lethal liver injury as comparedwith nontransgenic and hK8 WT mice ( $~$ 80% G61C vs. $~$ 40% control;Fig. 1 E). The increased lethality of G61C, as compared withWT mice, is caused by severe liver hemorrhage and apoptosis(Fig. 2 A). Although K8 G61C forms normal-appearing keratinfilaments under basal conditions, Fas administration causeshepatocyte drop-off and a more prominent keratin filament collapsein G61C, as compared with WT mice (Fig. 2 B). Fas administrationalso modulates K8/K18 phosphorylation (Ku et al., 2003), includingan increase in K8 S73/S431 and a decrease in K18 S33 phosphorylationin all transgenic lines (Fig. 2 C). However, K8 S73 hyperphosphorylation(Fig. 2 C) was significantly less in G61C, as compared withWT livers (65% less, as determined using quantitative blottingwith anti-K8 pS73 Ab; not depicted). The increased apoptosisin K8 G61C-expressing hepatocytes was also confirmed by enhancedformation of the caspase-generated K18 fragment (Fig. 2 C).Therefore, the natural K8 G61C mutation causes a dramatic increasein transgenic mouse susceptibility to stress-induced liver injury.

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Figure 2. K8 G61C accentuates Fas-induced liver injury. Livers were obtained from the indicated transgenic mice 4 h after PBS or Fas Ab administration. (A) Histological analysis (a–d) and TUNEL assay (a'–d') of transgenic mouse livers that were isolated after PBS (–) or Fas (+) intraperitoneal injection. Note the severe hemorrhage (H) and pyknotic nuclei in hK8 G61C (d and d') as compared with hK8 WT liver (b and b') after Fas administration. (B) Immunofluorescence staining of livers similar to those shown in A using an Ab that is specific to hK8. Note the similar staining pattern of hK8 WT and G61C livers under basal conditions (a and c), but the marked hepatocyte drop-off and the collapse of keratin filaments in G61C livers compared with WT mice after Fas injection (b and d). (C) Mouse livers were homogenized, followed by isolation of the total keratin pool by HSE. The extracts were separated by SDS-PAGE, and then visualized by Coomassie staining or blotting with Abs to the indicated epitopes. Each lane represents the analysis of one independent mouse liver. Bars: (A) 160 µm; (B) 40 µm.

Comparison of the effect of K8 and K18 mutation, or absence, in transfected cells and mouse livers
We compared the effect of K8 G61C (i.e., the patient-relatedvariant) and K18 R89C mutation, or K8/K18 absence in transfectedcells and mouse livers. K18 R89C is not a natural mutation,but K18 R89 is highly conserved among all IF proteins and thehomologous residue is a mutation "hotspot" in epidermal keratin-relateddiseases such as EBS (Porter and Lane, 2003). Overexpressionof K18 R89C in transgenic mice causes hepatocyte keratin filamentdisruption, hepatocyte fragility, and enhanced susceptibilityto liver injury and apoptosis (Ku et al., 1995, 2003) and wasthe major clue that led us to search for, and then associate,K8/K18 variants with human liver disease (Ku et al., 1997).When tested in transfected cells, K8 G61C behaves similarlyto K18 R89C (a control for Cys mutation); both are highly insolubleand generate keratin cross-links upon oxidative challenge whencompared with WT K8 and another natural K8 (R340H) variant (Fig. 3 A). The cross-linked K8 species are clearly detected in total lysates,but not cytosol (Fig. 3 A, lane 11 vs. 15), which indicatesthat most of these species are in the filament fraction. K8G61C insolubility (Fig. 3 B) and cross-linking after Fas orparaquat administration (Fig. 3 C) were similarly noted in transgenicmouse livers.

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Figure 3. K8 G61C decreases keratin solubility and promotes keratin cross-linking without altering hepatocyte fragility. (A) BHK cells were transiently cotransfected with the indicated mutant and/or WT keratins (K8 WT + K18 WT; K8 WT + K18 R89C; K18 WT + K8 G61C or R340H). After 3 d, cells were cultured in the presence or absence of 20 mM H₂O₂ for 1 h, and then divided into two portions. One portion was used to isolate a detergent-free cytosolic soluble fraction and the second to generate a total cell lysate. The isolates were subjected to SDS-PAGE under nonreducing conditions (to visualize cross-linked K8) and blotted with Abs specific to hK8 or hK18. Coomassie staining is also shown to demonstrate equal gel loading. Arrow indicates degraded K8. (B) Liver perfusion was used to isolate hepatocytes from hK8 WT and G61C mice. Total lysates and detergent-free cytosolic fractions were prepared from the isolated hepatocytes, followed by blotting with Abs specific to hK8, m/hK18, and mK18. Open arrows indicate degraded K8. (C) Oxidative stress or apoptosis was induced in mice by intraperitoneal administration of paraquat or Fas Ab, respectively. Total liver lysates were isolated and blotted with anti-hK8 Ab. Asterisk indicates nonspecific bands. Each lane represents the analysis of one independent mouse liver. (D) Total homogenates were prepared from livers of the indicated mouse genotypes (2 mice/genotype), followed by SDS-PAGE and blotting with Abs to the indicated proteins. A duplicate gel was stained with Coomassie blue to verify equal protein loading. Note that the K8 and K18 proteins are absent in both K8- and K18-null livers (lanes 3–6) because of degradation of the partner protein (Baribault et al., 1994; Magin et al., 1998). (E) Liver perfusion of K18-null, K18 R89C, K8 WT, and K8 G61C was performed to assess hepatocyte fragility. K18 R89C was used as a control and hepatocytes from these mice are already known to be fragile (Ku et al., 1995). Hepatocytes from K18-null and hK18 R89C livers had 16–24% viability (n = 3–6 livers/genotype), whereas hK8 WT and G61C hepatocytes had 82–89% viability (n = 4–6 livers/genotype). A summary of the phenotypes of transgenic mice that lack keratin expression (K8- and K18-null) or that express mutant K8 or K18 is shown. Shaded parameters are those examined in this study, whereas unshaded parameters represent summaries of previous studies (Marceau et al., 2001; Omary et al., 2002; Zatloukal et al., 2004).

We then assessed hepatocyte fragility and the expression ofseveral apoptosis-related proteins in K8 G61C mice as comparedwith K18 R89C, K8-, and K18-null mice. The K8- or K18-null mice,and K18 R89C mice, have a dramatically increased susceptibilityto liver injury and apoptosis (Marceau et al., 2001; Omary et al., 2002;Zatloukal et al., 2004). We examined the expression of severalapoptosis-associated proteins because c-Flip protein, but notmRNA, was reported to be absent in K8-null mouse liver, andc-Flip absence may account for the increased susceptibilityof K8-null livers to apoptosis (Gilbert et al., 2004). We didnot observe any difference in c-Flip (using two independentanti–c-Flip Abs) or several other apoptosis-associatedprotein levels between these four mouse groups and nontransgenicmouse groups (Fig. 3 D), which indicates that the previouslyreported results with c-Flip (Gilbert et al., 2004) were likelycaused by differences in Ab specificity.

We then examined hepatocyte fragility in K18-null, K8 WT, andK8 G61C mice upon liver perfusion because K8-null and the EBS-likeK18 R89C livers have remarkably fragile hepatocytes (Ku et al., 1995;Loranger et al., 1997). Nontransgenic and K18 R89C mice wereused as controls. Hepatocytes isolated from nontransgenic, K8WT, and K8 G61C livers had 82–89% (n = 4–6 livers/genotype)viability as compared with hepatocytes from K18-null livers,which had only 16–22% viability (n = 3). Hence, the phenotypesof keratin-null or keratin mutant genotypes (summarized in Fig. 3 E)suggest that K8 G61C alters hepatocyte function differentlythan when K18 is mutated at R89C or K8/K18 proteins are absent.This is despite the finding that both K18 R89C and K8 G61C decreasekeratin solubility and cause cross-linking during oxidativeconditions (Fig. 3, A–C).

K8 G61C disrupts K8 S73 phosphorylation by stress-activated kinases
Human K8 includes three major in vivo phosphorylation sites(S23/S73/S431) that are conserved in mouse K8 (Omary et al., 1998).S23 is phosphorylated under basal conditions, and S73/S431 arephosphorylated by SAPKs, such as p38, JNK, and p42 MAPK. p38phosphorylates only S73 and generates a unique, slightly slower-migratingK8 species (termed HK8) upon SDS-PAGE, whereas JNK and p42 phosphorylateS73/S431 and generate both HK8 and K8 phosphospecies (Fig. 4 A ;He et al., 2002; Ku et al., 2002). Given that the natural hK8G433S alters K8 S431 in vitro phosphorylation by p42 MAPK (Fig. 4 A;Ku et al., 2005; likely caused by proximity), we tested theeffect of several K8 mutations on K8 phosphorylation by p38/JNK/p42.K8 G61C blocks S73 phosphorylation by purified SAPKs, but doesnot completely eliminate S73 in vivo phosphorylation (likelyvia other kinases), as determined by blotting of transfected-celltotal lysates (Fig. 4 B) or transgenic mouse livers (Fig. 2 C)with anti-K8 pS73–specific Ab. Some of the other K8 mutantsalso inhibited K8 phosphorylation (R453C [all three kinases]and G433S [p42]), but the most prominent effect was noted inG61C (Fig. 4 B). Moreover, K8 I62V, which is a variant foundat higher frequency in controls as compared with liver diseasepatients (Ku et al., 2005), has similar S73 in vitro phosphorylationby the SAPKs as WT K8 (unpublished data). We further substantiatedthe effect of K8 G61C by comparing K8 S73 phosphorylation inBHK cells cotransfected with WT or kinase-inactive p38. K8 G61Ccauses the near-complete absence of K8 S73 phosphorylation bytransfected p38, which is similar to the near-absent phosphorylationof WT K8 upon kinase-inactive p38 transfection (Fig. 4 C). Hence,K8 G61C significantly inhibits K8 S73 phosphorylation in vivoby SAPKs.

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Figure 4. K8 G61C mutation disrupts K8 S73 phosphorylation in vitro and in vivo. (A) Schematic of K8 protein and its in vivo phosphorylation sites (Omary et al., 1998), and the distribution and frequency of K8 mutations associated with human liver disease (Ku et al., 2005). The rod domain of all IF proteins is divided into the following subdomains: IA, linker 1 (L1), IB, L12, and II. Positions of K8 phosphorylation (S23/S73/S431) and the relevant kinases are shown. K8 variants are highlighted by arrowheads, with each arrowhead representing an independent patient from the 467 liver explants that were studied; the single large arrowhead for R340H indicates 30 individuals (Ku et al., 2005). I465-fs is a frame-shift mutation at Ile465 that generates a truncated 468–amino acid protein (instead of 482). (B) BHK cells were transiently cotransfected with K18 WT and one of the indicated K8 constructs, followed by immunoprecipitation of K8/K18, then in vitro phosphorylation by p38, JNK, or p42 kinases. Labeled immunoprecipitates (ip) were analyzed by SDS-PAGE and radiography. HK8 and K8 in the radiograph represent K8 S73 and K8 S431 phosphorylation, respectively. Total lysates were also prepared from the transfected cells then blotted with Abs to the indicated epitopes. No band corresponding to K8 S431 phosphorylation was detected in the pS431 immunoblot of K8 G433S (lane 6) because of an alteration of the Ab epitope in the mutant. (C) BHK cells were triple-transfected with K8/K18 WT or K8 G61C/K18 WT, and WT or kinase-inactive p38 (AF mutant; T180A/Y182F). Total lysates were prepared and blotted with Ab to the indicated epitopes. Open arrows in B and C represent degraded K8.

K8 S73A predisposes to Fas-induced liver injury in transgenic mice
The effect of K8 G61C on S73 phosphorylation led us to hypothesizethat the inability to phosphorylate S73 in K8 G61C mice is amajor trigger for their increased susceptibility to apoptosis.We tested this hypothesis by generating transgenic mice thatoverexpress hK8 S73A and tested their predisposition to apoptosis.Expression of hK8 S73A was verified by blotting using anti-hK8–specificAb and by detection of K8 S73 phosphorylation, after Fas administration,in WT but not S73A hK8 livers (Fig. 5 A ). Fas administrationincreases K8 S431 phosphorylation in WT and S73A, but generatesthe K18 apoptotic fragment more prominently in S73A livers (Fig. 5 A).This suggests that inhibition of K8 S73 phosphorylation increasessusceptibility to Fas-mediated liver injury, which was confirmedby the marked lethality of S73A, as compared with WT K8 andnontransgenic mice (Fig. 5, B and C). The increased lethalityof K8 S73A mice is likely attributable to increased hemorrhageand apoptosis (Fig. 5 D), which mimics findings in K8 G61C mice(Fig. 2 A). K8 S73A and G61C mice share other features, includingnormal-appearing keratin filaments under basal conditions (Fig. 5 D),and similar cell viability of the isolated hepatocytes afterliver perfusion (84–92% viability; n = 5 livers).

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Figure 5. hK8 S73A transgenic mice have increased susceptibility to Fas-mediated hepatocyte apoptosis and injury. (A) Livers from nontransgenic (lane 1) and the indicated transgenic lines (lanes 2–9) were isolated from control or Fas-injected (± Fas) mice and analyzed as described in Fig. 2 C. Two independent transgenic lines per genotype (WT¹ and WT²; S73A¹ and S73A²) were used for the analysis (each of the lanes 2–9 represents one mouse from individual transgenic lines). (B and C) Nontransgenic FVB/n, hK8 WT, or S73A mice (19–30 age- and sex-matched mice per genotype) were injected with Fas and monitored as described in Fig. 1. Most deaths occurred within 12 h after Fas injection. The results are summarized in C. Mortality was significantly increased in hK8 S73A mice as compared with the combined (FVB/n + hK8 WT) mice. (D) Livers from Fas- or PBS-injected mice were analyzed by immunofluorescence staining (a–b'), by hematoxylin-eosin staining (c and c'), or TUNEL assay (d and d'). Hematoxylin-eosin staining and TUNEL assay of S73A livers under basal conditions (not depicted) were similar to those from the WT livers shown in Fig. 2 A (a and a'). H, hemorrhage. Bars: (a–b') 40 µm (c–d') 160 µm.

K8 G61C or S73A lead to sustained and enhanced phosphorylation of SAPK substrates after Fas-induced apoptosis
We hypothesized that G61C or S73A expression shunts phosphorylationfrom K8 S73 to other SAPK substrates after Fas stimulation.This hypothesis is based on the following: (a) cellular abundanceof K8 (e.g., prominent Coomassie staining; Fig. 1 B), (b) itsrole as an in vivo substrate for SAPKs (He et al., 2002; Ku et al., 2002),(c) compensatory down-regulation of endogenous mK8 (i.e., theconserved SAPK K8 S73 substrate [S79 in mK8]) in response tomutant/WT hK8 overexpression (Fig. 1 B and Fig. 2 C), and (d)inhibition of K8 S73 phosphorylation in K8 G61C. We tested thishypothesis by first showing that p42/44, JNK1/2, and p38 phosphorylation(and, hence, activation) were markedly but similarly increasedin response to Fas stimulation in WT and keratin mutant livers(Fig. 6 A ), which supports previous reports that SAPKs playproapoptotic roles (Gallo and Johnson, 2002; Kaplowitz, 2002;Baines and Molkentin, 2005). We then compared primary hepatocytecultures for their susceptibility to apoptosis by testing forthe presence of caspase-generated products after Fas stimulation(Fig. 6 B). The use of primary hepatocyte cultures eliminatesthe potential variability among mice and makes it feasible totest multiple time points. Cleaved caspases 3/7 were detectedbetween 3 and 5 h, but, as expected from the intact animal studies(Fig. 2 C and Fig. 5 A), the cleaved caspase products were moreevident in K8 G61C and S73A compared with WT hepatocytes (Fig. 6 B).

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Figure 6. Effect of K8 G61C or S73A mutation on SAPK activation and substrate phosphorylation. (A) Liver homogenates were obtained from the indicated transgenic mice (± Fas injection), separated by SDS-PAGE, and visualized by Coomassie staining (shown for equal loading) or by blotting with the indicated Abs. (B) Hepatocytes were isolated by liver perfusion then treated with 0.5 µg/ml Fas Ab for the indicated times. Total cell lysates were then prepared and analyzed as in A. (top) Lanes 1–12 represent samples loaded on the same gel, whereas lanes 13–18 were loaded on a separate gel. (bottom) Representative samples from the top panel that were analyzed on the same gel to confirm the relative changes in caspase cleavage. (C) Total lysates of primary hepatocytes were prepared and analyzed as in B. Arrows likely represent degradation products. Note that phosphorylation of the SAPK substrates, c-Jun, CREB, and p90RSK, is increased and is more sustained in K8 G61C or S73A hepatocytes as compared with K8 WT hepatocytes.

Finally, we compared the phosphorylation of endogenous mouseproteins that are known to serve as SAPK substrates: c-Jun (S63/S73)by JNK, cAMP response element binding protein (CREB) and NF- ${kappa}$ Bp65 by p38, and p90RSK by p42/44 (Deak et al., 1998; Roux and Blenis, 2004;Liu and Lin, 2005). Although phosphorylation of NF- ${kappa}$ B p65 wassimilar in K8 WT, G61C, or S73A hepatocytes after Fas treatment,phosphorylation of c-Jun, CREB, and p90RSK in K8 G61C and S73Ahepatocytes was more pronounced and sustained when comparedwith WT hepatocytes (Fig. 6 C). The pattern of phosphorylated/activatedSAPKs in K8 WT, G61C, or S73A hepatocytes after Fas treatmentis relatively similar (Fig. 6 C), and activation by Fas is notas dramatic in primary cultures as it is in vivo (e.g., lanes1 and 2 for phospho-JNK in Fig. 6 C, as contrasted with Fig. 6 A),which is likely caused by the stress incurred upon hepatocyteisolation. Our data support the conclusion that increased phosphorylationof nonkeratin SAPK substrates in G61C and S73A hepatocytes reflectsa shunting of phosphorylation toward these other substratesin association with caspase activation.

Discussion

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Abstract
Introduction
Results
Discussion
Materials and methods
References

Disease relevance
The findings herein represent the first in vivo evidence thatnaturally occurring human K8 mutations can predispose to liverinjury and apoptosis. Our results show that introducing hK8G61C into mice predisposes to liver injury and apoptosis, andsuggest the following sequence of events in response to stress:a G61C-mediated conformational change leads to the inabilityof K8 S73 to serve as a SAPK substrate, which creates an imbalanceof kinase substrate availability, thereby predisposing to apoptosisand liver injury (Fig. 7 ). K8 G61C is the second most frequentliver disease–associated variant after R340H (Ku et al., 2005;Strnad et al., 2006a). Mutations of IF proteins, including keratins,desmin, neurofilaments, and lamins, among others, are associatedwith a wide range of tissue-specific human diseases (Fuchs and Cleveland, 1998;Omary et al., 2004). Compared with most other IF mutations,one unique characteristic of K8/K18 mutations is that they posea risk of disease, rather than directly causing it (Omary et al., 2002;Porter and Lane, 2003; Ku et al., 2005). The results hereinfill an important missing link by experimentally demonstratingthat a human disease-associated keratin mutation can, indeed,cause disease when an animal carrying the mutation is challengedby oxidative and other stresses. Therefore, the findings inK8 G61C transgenic mice provide strong supporting evidence forthe human association studies that have been performed to date.

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Figure 7. K8 mutation shunts keratin phosphorylation by stress-activated kinases. During stress, activated kinases such as p38 MAPK phosphorylate K8 S73 and other proapoptotic substrates. However, K8 G61C mutation interferes with the ability of the highly abundant K8 S73 to serve as a substrate, which renders other substrates available for potential phosphorylation and consequent rapid progression of apoptosis. Filled dots indicate phosphorylated residues. The phosphate sponge model works in a hepatocyte-protective fashion in livers that express WT K8 and provides a function for K8 S73 phosphorylation that becomes unmasked upon K8 G61C mutation. This model predicts that keratins (and possibly other IFs) undergo hyperphosphorylation in part to absorb, in a "bulk" fashion given their abundance, cell kinase activation. Such sponge activity can be beneficial (e.g., K8 S73), or potentially detrimental, in a phosphorylation site-specific and context-dependent fashion. This model provides one (of several potential) nonmechanical functional capability for IFs and their phosphorylation and does not exclude the possibility that some kinase substrates may undergo dephosphorylation (e.g., via phosphatase activation by phosphorylation) and that other phosphorylation-dependent or -independent mechanisms for protection may be involved.

The mechanisms of liver injury predisposition by different K8/K18variants may be variant/disease-specific or may have mechanisticoverlap. This is supported by the inability of other (non-G61C)K8 natural mutants (e.g., G52V, Y53H, I465-fs [Fig. 4 B], andI62V [not depicted]) to interfere with SAPK phosphorylationof K8. Furthermore, K18 R89C (in mice) alters a K8/K18 mechanicalfunction (i.e., fragility predisposition) that is not sharedby K8 G61C (Fig. 3 E). K18 R89C also primes hepatocytes to undergoapoptosis (Ku et al., 2003) and oxidative injury (Zhou et al., 2005),which are likely mechanisms that are shared by K8 G61C and K8S73A. A common denominator for imparting protection from liverinjury is keratin phosphorylation, which correlates with progressionfrom chronic to end-stage liver disease (Toivola et al., 2004;Zatloukal et al., 2004). This notion is supported by the findingthat K18 S52A (S52 is a major hK18 phosphorylation site) expressionpredisposes to hepatotoxic injury in transgenic mice (Ku et al., 1998),and by the results herein.

Relationship between K8 G61 mutation and S73 phosphorylation
The conformational link between K8 S73 phosphorylation and G61is supported by the similar findings in K8 G61C and S73A mice,and by the inhibition of K8 S73 phosphorylation in vitro uponG61C mutation. This link is also supported by inhibition ofbinding of an Ab directed to a K8 G61C-containing epitope whenS73 is phosphorylated (Tao et al., 2006). Immunoblotting ofliver homogenates from transgenic mice with this Ab showed itsbinding with WT and S73A, but not with G61C K8 homogenates (Fig.S1, available at http://www.jcb.org/cgi/content/full/jcb.200602146/DC1).K8 S73 phosphorylation also leads to a distinct retardationin migration during SDS-PAGE, which is specific to that phosphorylationsite and is also seen when S73 is mutated to aspartate (Liao et al., 1997;Ku et al., 2002). Hence, the phenotype we observe appears tobe caused by mutation-related interference with a kinase–substrateinteraction though other direct/indirect interference with potentialstable keratin and kinase–kinase regulator interactionsis possible. For example, p38 and JNK associate with keratins,but this association appears to be stoichiometrically limitedand is more consistent with a kinase–substrate association(He et al., 2002; Ku et al., 2002). In addition, both WT andS73A K8 coimmunoprecipitate with p38 MAPK, although we couldnot adequately test the K8 G61C mutant because of its limitedsolubility in mild detergents (unpublished data). Further supportfor a conformational link between K8 G61C and S73 phosphorylationis that the G61C mutation inhibits in vitro phosphorylationof K8 S73 by purified SAPKs, but does not significantly affectK8 S431 phosphorylation (Fig. 4 B).

Lack of accessibility of SAPKs to K8 S73 upon G61C mutationmay also be impacted by the formation of K8 cross-links in responseto oxidative stress (Ku et al., 2001; Owens et al., 2004). Inthis context, exposure to Fas or paraquat increases K8 cross-linkedspecies that are otherwise barely detectable (Fig. 3 C). Thisreflects the change in the normally reducing cytoplasmic environmentunder stress, with production of reactive oxygen species duringFas-mediated apoptosis and other oxidative stresses as seenin rat hepatocytes (Reinehr et al., 2005) and T cell lines (Sato et al., 2004).The effect of G61C on keratin solubility (Fig. 3, A and B) mayalso independently contribute to kinase inaccessibility.

K8 S73 phosphorylation is likely to be associated with severalfunctions because it occurs during stress, apoptosis, and mitosis(Liao et al., 1997; Ku et al., 2002; Toivola et al., 2002).Previous studies in transfected cells (Ku et al., 2002) showedthat K8 S73 phosphorylation promotes keratin filament reorganization(e.g., Ala substitution blocked stimulus-induced filament reorganization,which was rescued by Asp substitution). The multiplicity ofkeratin phosphorylation sites raises the untested possibilitythat site-specific phosphorylation can have a domino effectthat "opens" the filaments to additional phosphorylation/dephosphorylationevents, with consequent functional implications.

The phosphate sponge model
The similarity of the K8 G61C and S73A transgenic mice phenotypessupports an important role for S73 as a phosphate sponge forSAPKs in normal tissues undergoing stress. Amongst the earliestdescriptions of IFs potentially serving as "phosphate sinks"was the observation of significant vimentin and keratin hyperphosphorylationafter short exposure of cells to okadaic acid (Lai et al., 1993).Subsequent studies suggested that neurofilaments may serve asphosphate sinks (Nguyen et al., 2001), which was supported byothers, although in this case the sink model is not protective,as initially hypothesized (Lobsiger et al., 2005). We electedto use the term "sponge" instead of sink because it is moregeneral, in that sponges are more easily transportable (i.e.,dynamic) and not only collect spills but also allow their recovery(as free phosphates) with ready availability of fresh spongecapacity. We hypothesize that a phosphorylation sponge effect(Fig. 7) may be detrimental or beneficial, in a context andphosphorylation site-specific fashion, and that in the caseof K8 S73 the phosphorylation role is beneficial. This modeldoes not exclude the possibility that some antiapoptotic kinasesubstrates may in fact become hypophosphorylated, but predictsthat overall phosphorylation is shunted, with the net effectbeing enhanced apoptosis.

The abundance of cytoplasmic keratins allows for plentiful spongecapacity. For example, K8/K18 can be easily seen by Coomassiestaining upon HSE (Fig. 1 B), and they make up 5% of culturedcolonocyte total proteins (Omary et al., 1998) and 0.2% of totalmouse liver protein (Zhong et al., 2004; the 0.2% is an underestimatebecause it includes proteins from other resident nonkeratin-containingendothelial and Kupffer cells and some blood proteins). Also,K8 S73 is a unique and readily available SAPK substrate becauseit behaves as a switch that is either "on" or "off," being completelyunphosphorylated (off) under basal conditions but turning onvia phosphorylation during apoptosis and cell injury (Liao et al., 1997).

SAPKs can play proapoptosis roles in several disorders, includingliver (Kaplowitz, 2002), neuronal (Gallo and Johnson, 2002),and cardiac (Baines and Molkentin, 2005) disease. For example,disruption of JNK3 in mice results in resistance to excitotoxicity-inducedneuronal apoptosis (Yang et al., 1997) and pharmacologic inhibitionof p38 interferes with TNF-induced hepatocyte apoptosis (Pastorino et al., 2003).Most of the known SAPK substrates are signaling molecules, suchas protein kinases (e.g., MSKs, RSKs, and MNKs), transcriptionfactors (e.g., c-Jun, Elk-1, c-Fos, and NF- ${kappa}$ B), or apoptosis-associatedproteins (e.g., Bim and Bad; Roux and Blenis, 2004; Liu and Lin, 2005).Some protein kinases are phosphorylated and activated by SAPKsand then phosphorylate and activate transcription factors amongother substrates. For example, p38 MAPK phosphorylates MSK1that can phosphorylate the CREB transcription factor (Deak et al., 1998).The increased phosphorylation of cellular proteins after Fasstimulation was not universal in G61C and S73A hepatocytes (e.g.,phospho–NF- ${kappa}$ B p65 was not altered; Fig. 6 C). Several othersubstrates were tested, including MSKs, Elk-1, c-Fos, c-Myc,p53, and Bim, but the results were unrevealing because of thelack of cross reactivity of the respective Abs with mouse proteins(unpublished data). The K8 G61C/S73A-associated increase inc-Jun phosphorylation supports the enhanced susceptibility ofG61C and S73A hepatocytes toward apoptosis, given that AP-1members such as c-Jun are involved in proapoptotic or survivalsignaling depending on the cellular context and external stimulus.For example, stress-activated JNK phosphorylates c-Jun, whichresults in enhanced transcription of target genes (e.g., FasL)associated with apoptosis (Hess et al., 2004), and c-Jun S63/73mutations in mice protects neurons from apoptosis (Behrens et al., 1999).The role of CREB and p90RSK is well studied in cell survival,but less so in proapoptotic pathways. However, serial analysisof chromatin occupancy supports the involvement of CREB in severalproapoptotic gene products such as DEDD, TRADD, GADD45 ${gamma}$ , andBim (Impey et al., 2004).

Implications based on the relative conservation of K8 S73
Several type II keratins contain a unique LLS/TPL motif, whichis ⁷¹LLSPL in hK8 (i.e., S73-containing) or LLTPL in K4/K5/K6and hair keratins (Liao et al., 1997; Toivola et al., 2002).LLS/TPL is phosphorylated during apoptosis and other stressesby SAPKs in several epithelial tissues, including the liverand intestine (K8) and the esophagus and skin (K4/K5/K6; Liao et al., 1997;Ku et al., 2002; Toivola et al., 2002). Our findings suggestan important nonmechanical role for K8 in protecting hepatocytesfrom injury by serving as a phosphate sponge for SAPKs thatcan absorb some of their untoward effects (Fig. 7). This rolemay extend to keratins and their related diseases in other tissueswhere the K8 S73-containing LLS/TPL motif is conserved, andis negatively impacted by G61C mutation and possibly other K8or K18 liver disease–associated mutations.

Materials and methods

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Abstract
Introduction
Results
Discussion
Materials and methods
References

Reagents and keratin-null mice
The reagents used include the following: MLR (Alexis Corp.),paraquat (Sigma-Aldrich), TdT-FragEL DNA fragmentation detectionkit (Calbiochem), p38 ${alpha}$ MAPK (Upstate Biotechnology), JNK andp42 MAPK (Cell Signaling Technology), collagenase type II (WorthingtonBiochemical Corp.), and Lipofectamine (Invitrogen). All Absto keratins and phosphokeratins were previously described (Ku et al., 2004).Other Abs used were directed to Fas for mouse injection (BDBiosciences); to phospho- or nonphospho-p38, CREB, CREB pS133,p90RSK, phospho-p90RSK (human T359/S363 and mouse T348/S352),phospho-NF- ${kappa}$ B p65 (human S536 and mouse S534), phospho-p42, JNK,and c-Jun (Cell Signaling Technology); to Fas for immunoblotting,FADD, and Bax (Upstate Biotechnology); and to Fas-ligand, nonphospho–c-Jun(Santa Cruz Biotechnology, inc.). Two independent Abs were usedto detect mouse c-Flip; one directed to an NH₂-terminal region(SAEVIHQVEEALDTDE) that is 100% identical in human and mousec-Flip (Upstate Biotechnology), and another directed to a mouse-specificCOOH-terminal region (DKVYAWNSGVSSKEKYS) of c-Flip (Sigma-Aldrich).K8- and K18-null mice were provided by R. Oshima (The BurnhamInstitute, La Jolla, CA) and T. Magin (University of Bonn, Bonn,Germany), respectively.

Transgene constructs and generation of transgenic lines
A transformer kit (CLONTECH Laboratories) was used to introducesingle point mutations into a human (h) WT 12-kb genomic K8clone (Krauss and Franke, 1990). The K8 genomic clone (providedby W. Franke, German Cancer Research Center, Heidelberg, Germany)includes endogenous regulatory elements that maintain tissueexpression. Two mutant genomic constructs were generated (hK8G61C or S73A), and both strands of the mutated region were sequencedto confirm the mutation. Fidelity of the mutant and WT constructswas verified by testing its expression by transient transfectioninto BHK cells. The 12-kb Sal I fragments of mutant or WT genomichK8 DNA were then injected into pronuclei of fertilized FVB/nmouse eggs. Progeny mice carrying the hK8 transgene were chosenafter PCR screening of tail genomic DNA, which was followedby breeding to select for germline transmission (primers ofa 250-bp PCR fragment; 5'-GGCGGCGGCTATGGTGGGGCC-3' and 5'-AGATGTGCATAGGGACCGGGA-3').Two independent heterozygous mouse lines per construct wereestablished and expanded (K8: WT¹ and WT²; G61C¹ and G61C²;and S73A¹ and S73A²), all in an FVB/n background, and then usedfor subsequent studies. The two transgenic lines for each constructhad similar K8 expression and afforded near-identical results.

Toxin administration and hepatocyte isolation
For the lethality experiments, mice (age and sex matched) werefasted overnight, followed by intraperitoneal injection of FasAb (0.15 µg/g mouse body weight) or MLR (30 ng/g mousebody weight; Ku et al., 2004). Mice were killed by CO₂ inhalation4 h after Fas Ab injection, and their livers were isolated andprocessed for immunofluorescence, histology (HistoTec Laboratories),and TUNEL analyses (Ku et al., 2004). For induction of oxidativeinjury, mice were fasted overnight then injected intraperitoneallywith paraquat (70 µg/g mouse body weight; Holzenberger et al., 2003),followed by harvesting of livers after 60 h. Hepatocyte isolationwas performed by liver perfusion of three to six age- and sex-matchedmice/genotype, using collagenase type II (Ku et al., 1995).Cultured hepatocytes were treated with Fas Ab (0.5 µg/mlfor 0.5–5 h), followed by preparation of cell lysatesfor immunoblotting.

Biochemical and immunologic analyses
Keratins were isolated by HSE using liver pieces as previouslydescribed (Ku et al., 2004). Alternatively, total liver homogenateswere prepared by solubilizing in SDS-containing buffer. Proteinswere separated by SDS-PAGE, followed by staining with Coomassieblue or transferal to membranes; they were then immunoblottedand visualized by enhanced chemiluminescence. Quantitative immunoblottingwas performed using serial dilutions of the two samples to becompared and analyzed on the same gel. Immunofluorescence stainingwas done as previously described (Ku et al., 2004), and fluorescenceimages were analyzed using a confocal microscope (MRC 1024ES;Bio-Rad Laboratories).

Solubility analysis and in vitro phosphorylation
BHK cells were transiently cotransfected (using Lipofectamine)with K18 WT and K8 (WT or mutant constructs; Ku et al., 2005)or K18 R89C and K8 WT (Ku et al., 1995). 3 d after transfection,the cells were further cultured (37°C) in the presence orabsence of 20 mM H₂O₂ for 1 h, followed by isolation of a detergent-free,cytosolic soluble fraction or a total cell lysate (Ku et al., 2005).The triple transient transfections with kinase active/inactivep38 ${alpha}$ and keratins were also performed in BHK cells (Ku et al., 2002).

In vitro phosphorylation was done as previously described (Ku et al., 2004).K8/K18 immunoprecipitates, which were isolated from BHK-transfectedcells, were washed with kinase-specific buffers (Cell SignalingTechnology; Upstate Biotechnology), heated (90°C) to inactivateany bound kinase activity, and incubated with the kinases (p38,JNK, or p42) and ${gamma}$ -[³²P]ATP (Ku et al., 2004). Kinase reactionswere quenched by boiling in the presence of 2% SDS-containingbuffer, which was followed by analysis by SDS-PAGE and autoradiography.

Online supplemental material
Fig. S1 shows blotting with anti-hK8 G61C Ab that binds withWT and S73A, but not G61C K8, in transgenic liver homogenates.Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200602146/DC1.

Acknowledgments

We are grateful to the generous contributions of reagents andmice that were provided by Drs. Werner Franke (human K8 genomicclone), Robert Oshima (K8-null mice), and Thomas Magin (K18-nullmice); to Steve Avolicino (HistoTec Laboratory) for the histochemicalstaining; to Evelyn Resurreccion for assistance with tissuestaining; and to Kris Morrow for helping with figure preparation.

This work was supported by National Institutes of Health (NIH)DK47918 and VA Merit awards (M.B. Omary). N-O. Ku was supported,in part, by a Veterans Administration Research Enhancement AwardProgram, and NIH Digestive Disease Center grant DK56339 PilotAward.

The authors declare no competing financial interests.

Submitted: 24 February 2006

Accepted: 26 May 2006

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