Mtu1-Mediated Thiouridine Formation of Mitochondrial tRNAs Is Required for Mitochondrial Translation and Is Involved in Reversible Infantile Liver Injury

Yong Wu; Fan-Yan Wei; Layla Kawarada; Takeo Suzuki; Kimi Araki; Yoshihiro Komohara; Atsushi Fujimura; Taku Kaitsuka; Motohiro Takeya; Yuichi Oike; Tsutomu Suzuki; Kazuhito Tomizawa

doi:10.1371/journal.pgen.1006355

Abstract

Reversible infantile liver failure (RILF) is a unique heritable liver disease characterized by acute liver failure followed by spontaneous recovery at an early stage of life. Genetic mutations in MTU1 have been identified in RILF patients. MTU1 is a mitochondrial enzyme that catalyzes the 2-thiolation of 5-taurinomethyl-2-thiouridine (τm⁵s²U) found in the anticodon of a subset of mitochondrial tRNAs (mt-tRNAs). Although the genetic basis of RILF is clear, the molecular mechanism that drives the pathogenesis remains elusive. We here generated liver-specific knockout of Mtu1 (Mtu1^LKO) mice, which exhibited symptoms of liver injury characterized by hepatic inflammation and elevated levels of plasma lactate and AST. Mechanistically, Mtu1 deficiency resulted in a loss of 2-thiolation in mt-tRNAs, which led to a marked impairment of mitochondrial translation. Consequently, Mtu1^LKO mice exhibited severe disruption of mitochondrial membrane integrity and a broad decrease in respiratory complex activities in the hepatocytes. Interestingly, mitochondrial dysfunction induced signaling pathways related to mitochondrial proliferation and the suppression of oxidative stress. The present study demonstrates that Mtu1-dependent 2-thiolation of mt-tRNA is indispensable for mitochondrial translation and that Mtu1 deficiency is a primary cause of RILF. In addition, Mtu1 deficiency is associated with multiple cytoprotective pathways that might prevent catastrophic liver failure and assist in the recovery from liver injury.

Author Summary

Mitochondrial transfer tRNA (mt-tRNA) contains a variety of chemical modifications that are introduced post-transcriptionally. Three mt-tRNAs for Lys, Gln and Glu contain 5-taurinomethyl-2-thiouridine (τm⁵s²U) in their anticodons. It is known that the loss of 2-thiolation of τm⁵s²U is strongly associated with the development of reversible infantile liver failure (RILF) because pathogenic mutations of RILF were found in the MTU1 gene, which encodes an enzyme responsible for the 2-thiolation of τm⁵s²U. However, the molecular mechanism underlying RILF pathogenesis associated with a lack of MTU1 remains elusive. To understand the physiological function of MTU1 and its association with liver failure, we generated liver-specific Mtu1-deficient (Mtu1^LKO) mice. Mtu1 deficiency abolished 2-thiouridine formation in the three mt-tRNAs. Loss of the 2-thiouridine modification resulted in a marked impairment of mitochondrial translation and abnormal mitochondrial structure. Consequently, the Mtu1^LKO mice exhibited liver injury, which resembles the symptoms of RILF patients. Furthermore, mitochondrial dysfunction in Mtu1^LKO mice induced mitochondrial biogenesis and suppressed oxidative stress. These findings elucidate the cellular and physiological functions of Mtu1 and provide a mouse model for understanding RILF pathogenesis.

Citation: Wu Y, Wei F-Y, Kawarada L, Suzuki T, Araki K, Komohara Y, et al. (2016) Mtu1-Mediated Thiouridine Formation of Mitochondrial tRNAs Is Required for Mitochondrial Translation and Is Involved in Reversible Infantile Liver Injury. PLoS Genet 12(9): e1006355. https://doi.org/10.1371/journal.pgen.1006355

Editor: Nils-Göran Larsson, Max Planck Institute for Biology of Ageing, GERMANY

Received: May 19, 2016; Accepted: September 8, 2016; Published: September 30, 2016

Copyright: © 2016 Wu et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Data Availability: All relevant data are within the paper and its Supporting Information files.

Funding: This work was supported by a Grant-in-aid for Scientific Research from the Ministry of Education, Culture, Sports, Science and Technology of Japan, by the Japan Agency for Medical Research and Development, by the Japan Science and Technology Agency, by the Takeda Science Foundation, and by a scholarship from the China Scholarship Council. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Competing interests: The authors have declared that no competing interests exist.

Introduction

Transfer RNA (tRNA) is an adaptor molecule that converts genetic information into an amino acid sequence in protein synthesis. tRNAs contain a wide variety of modified nucleosides that are introduced post-transcriptionally [1, 2]. In mammalian mitochondria, 22 subtypes of tRNAs encoded in mitochondrial DNA participate in the translation of 13 protein subunits of respiratory chain complexes in mitochondria. Fifteen species of modified nucleotides are found at 118 positions of bovine mitochondrial tRNAs (mt-tRNAs) [3]. A number of pathogenic point mutations associated with mitochondrial diseases are found in mt-tRNA genes [4–5]. Some of these mutations impair mt-tRNA modifications, leading to defective translation and mitochondrial dysfunction. In addition, a number of pathogenic mutations have been found in mt-tRNA-modifying enzymes, including MTO1 [6–8], GTPBP3 [9], MTU1 [10–13], and PUS1 [14], indicating that decreased modifications of mt-tRNAs caused by tRNA mutations and defective tRNA-modifying enzymes result in pathological consequences. Supporting these findings, the physiological roles of tRNA-modifying enzymes have been extensively studied in mouse models lacking mt-tRNA-modifying enzymes [15–16].

Unique to mitochondrial tRNA modifications, 5-taurinomethyluridine (τm⁵U) is present at the first position of the anticodon (i.e., the “wobble position” or position 34) of mt-tRNAs for Leu (UUR) and Trp, whereas its 2-thiouridine derivative (τm⁵s²U) is found at the same position of mt-tRNAs for Glu, Gln and Lys [17–18]. These modifications allow mt-tRNAs to recognize their cognate codons precisely and ensure accurate translation in the mitochondria. The enzymes mitochondrial tRNA translation optimization 1 (Mto1) and GTP binding protein 3 (Gtpbp3) are assumed to be responsible for τm⁵U formation [19]. In addition, mitochondrial tRNA-specific 2-thiouridylase 1 (MTU1) catalyzes the 2-thiolation of τm⁵U to form τm⁵s²U [19].

The lack of a yeast homolog of MTU1 resulted in impaired mitochondrial translation activity and a severe respiratory defect [19]. Moreover, acute knockdown of MTU1 in HeLa cells reduced the oxygen consumption rate and resulted in a defective mitochondrial membrane potential [19]. Intriguingly, MTU1 has been implicated in the pathogenesis of reversible infantile liver failure (RILF) [10–13], a life-threatening condition characterized by acute liver dysfunction during the first 2–4 months after birth. However, a majority of patients spontaneously recover and never exhibit another symptom [20]. Genomic analysis has identified a variety of autosomal recessive mutations, including substitutions, insertions and deletions, in the coding region of MTU1 in RILF patients [20]. These mutations in MTU1 are predicted to cause the loss of MTU1 activity, which subsequently triggers the pathological symptoms. Indeed, immortalized cell lines derived from RILF patients exhibit very low levels of MTU1 with a marked reduction of 2-thiolation levels in mt-tRNAs, leading to defective mitochondrial translation [21]. However, little reduction of mitochondrial translation has been observed in the fibroblasts of RILF patients [22], which raised some discrepancies by different groups regarding the observed MTU1 functions.

To reveal the physiological role of MTU1-mediated 2-thiouridine formation of τm⁵s²U in the regulation of mitochondrial protein translation in hepatocytes and its relevance in RILF, we generated multiple lines of conditional Mtu1 knockout mice and investigated the molecular functions of Mtu1 in these murine models.

Results

Mtu1 is indispensable for embryonic development

To investigate the physiological role of Mtu1, we generated constitutive Mtu1 knockout mice (Mtu1^-/-) (Fig 1A). However, no Mtu1^-/- mice were obtained after multiple generations of breeding (Fig 1B). The embryos at 9 days post-coitum (E9) were isolated for morphological examination. While the morphology of Mtu1^+/- embryos did not differ from that of Mtu1^+/+ embryos, the size of Mtu1^-/- embryos was strikingly small (Fig 1C and 1D). To visualize the internal structure, the embryos were stained with platelet endothelial cell adhesion molecule-1 (PECAM-1). Mtu1^+/+ and Mtu1^+/- embryos exhibited organized blood vessel networks that surrounded well-developing tissues, such as the heart, brain and spinal cord (Fig 1E). In contrast, neither blood vessel networks nor developmental stage-matched tissues were observed in Mtu1^-/- embryos (Fig 1E). Considering these morphologies, we concluded that the Mtu1^-/- embryo died at a developmental stage as early as E7.5~8.

Download:

Fig 1. Mtu1 is essential for embryonic development.

(A) Breeding strategy to generate constitutive Mtu1 knockout mice. ATG indicates the start codon. (B) Total number of wild-type (Mtu1^+/+), heterozygous (Mtu1^+/-) and homozygous (Mtu1^-/-) animals obtained from parental Mtu1^+/- mice. (C) Morphology of Mtu1^+/+, Mtu1^+/- and Mtu1^-/- embryos at stage E9. Bar = 5 mm. Note that the development of Mtu1^-/- embryos was severely delayed. (D) Genotyping analysis of embryos. DNA fragments corresponding to the wild-type (WT) allele and deleted (KO) allele are shown. Asterisks indicate the genotypes of the embryos shown in (C). (E) Blood vessel networks in embryos shown in (C) were examined by immunostaining against PECAM-1.

https://doi.org/10.1371/journal.pgen.1006355.g001

Liver-specific Mtu1 knockout mice exhibited liver injury and altered metabolism

To avoid the embryonic lethality, we generated liver-specific Mtu1 knockout mice (Mtu1^LKO) (S1 Fig). The Mtu1^LKO mice were viable and developed without any obvious morphological defects (S1 Fig). We confirmed a 10-fold reduction in the Mtu1 transcript levels in the liver of Mtu1^LKO mice compared to Mtu1^Flox mice (Fig 2A). The average body weight of Mtu1^LKO mice did not differ from that of Mtu1^Flox mice (Fig 2B). Laboratory examinations of 3-week-old mice revealed significantly elevated plasma levels of lactate, aspartate aminotransferase (AST) and alanine aminotransferase (ALT) in Mtu1^LKO mice (Fig 2C–2E). In addition, the Mtu1^LKO mice exhibited a high level of serum lactate dehydrogenase (LDH) and a low level of albumin (ALB) compared to the Mtu1^Flox mice (Table 1). These results clearly indicate that liver injury occurs in the Mtu1^LKO mice. Interestingly, the Mtu1^LKO mice exhibited altered metabolism. The levels of total cholesterol (T-CHO), high-density lipoprotein cholesterol (HDL-C), amylase (AMY), creatinine (CRE) and calcium (Ca) were significantly reduced in the Mtu1^LKO mice (Table 1). In agreement with these biochemical results, a gene expression analysis revealed an increase in the expression levels of genes involved in glycolysis (Glucokinase, Gck), gluconeogenesis (Glucose-6-phosphatase catalytic subunit, G6pc), and lipid oxidation (carnitine palmitoyltransferase 2, Cpt2) in the Mtu1^LKO mice (Fig 2F).

Download:

Fig 2. Hepatocyte-specific Mtu1 knockout mice exhibited liver injury and altered metabolism.

(A) Relative expression levels of Mtu1 in liver tissues of control (Flox) and Mtu1^LKO (LKO) mice. n = 3 each. ****P<0.0001. (B) The body weight of male mice at 3 weeks of age. n = 3 each. (C-E) Plasma lactate (C), aspartate aminotransferase (AST) (D) and alanine aminotransferase (ALT) (E) of Mtu1^LKO and control male mice at 3 weeks of age. n = 6 each. *P < 0.05, ****P < 0.0001. (F) Expression levels of selected metabolism-related genes in the livers of Mtu1^LKO and control male mice at 3 weeks of age were examined by quantitative PCR (n = 4 each). The relative expression levels are shown as a heat map. *P <0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001.

https://doi.org/10.1371/journal.pgen.1006355.g002

Download:

Table 1. Serum biochemical data of Mtu1^Flox and Mtu1^LKO mice.

https://doi.org/10.1371/journal.pgen.1006355.t001

We next investigated liver injury in the Mtu1^LKO mice at the histological level. The Mtu1^LKO mice exhibited normal liver structures compared to Mtu1^Flox mice (S1 Fig). No obvious fibrosis was observed in the livers of Mtu1^LKO mice by Masson trichrome staining (Fig 3A and 3B). Interestingly, there was an infiltration of macrophages (arrows in Fig 3C and 3D) and spotty necrosis (arrows in Fig 3E) in the livers of Mtu1^LKO mice. In addition, enlarged hepatocytes with karyomegaly and multiple nuclei were observed in the Mtu1^LKO mice (arrows in Fig 3F). These histological features of Mtu1^LKO mice resemble the clinical features of RILF patients [20].

Download:

Fig 3. Hepatocyte-specific Mtu1 knockout mice exhibited liver injury.

(A-B) Masson trichrome staining of liver sections from Flox and LKO mice. Bars = 0.2 mm. (C-F) High magnification views of representative H&E staining of liver sections from Flox (C) and LKO (D-F) mice. Bars in panels v-viii = 0.05 mm. (D) Representative macrophage infiltration (arrows) in an LKO mouse liver section. (E) Representative spotty necrosis (arrows) in an LKO mouse liver section. (F) Representative hepatocytes with karyomegaly (arrows) and multiple nuclei (arrowhead) in an LKO mouse liver section.

https://doi.org/10.1371/journal.pgen.1006355.g003

Mtu1-mediated s² modification is essential for mitochondrial translation

To clarify the molecular function of Mtu1 and its association with liver injury, we examined mt-tRNA modifications and mitochondrial translation in Mtu1-deficient hepatocytes. mt-tRNA^Gln, mt-tRNA^Glu and mt-tRNA^Lys were individually purified from liver tissues and subjected to mass spectrometry analysis. Interestingly, these mt-tRNAs were partially s²-modified even in the livers of Mtu1^Flox mice; 40~70% of the mt-tRNA^Glu, mt-tRNA^Gln and mt-tRNA^Lys contained τm⁵s²U and s²U modifications, whereas the remaining 30~60% of the mt-tRNA contained τm⁵U modifications and unmodified U (S2 Fig). In the livers of Mtu1^LKO mice, the s² modification was nearly absent in the three mt-tRNAs (Fig 4A–4C). There was a trace of τm⁵s²-containing mt-tRNAs, but this result was most likely derived from non-hepatic cells. Notably, the level of τm⁵U in mt-tRNA^Glu, mt-tRNA^Gln and mt-tRNA^Lys remained unchanged despite of the loss of the s² modification (S2 Fig). In addition to mitochondrial s² modification, we examined other sulfur-containing modifications, including mcm⁵s²U (5-methoxycarbonylmethyl-2-thiouridine) modification in cytosolic tRNAs and ms²i⁶A (2-methylthio-N6-isopentenyladenosine) modification in mt-tRNAs. Interestingly, the abundance of these modifications was up-regulated in the livers of Mtu1^KO mice compared to Mtu1^Flox mice (S3 Fig).

Download:

Fig 4. Loss of s² modification in Mtu1-deficient liver.

(A-C) Representative mass chromatograms of mt-tRNA^Gln (A), mt-tRNA^Glu (B) and mt-tRNA^Lys (C) purified from the livers of control (Flox) and knockout (LKO) mice. Arrowheads indicate traces of fragments containing s² modification in LKO mice. Note that the levels of s²-containing mt-tRNAGln, mt-tRNAGlu and mt-tRNALys were almost absent in LKO mice. n.d.: not detected. n.d.: not detected.

https://doi.org/10.1371/journal.pgen.1006355.g004

Next, we examined mitochondrial protein translation in primary hepatocytes isolated from Mtu1^LKO and Mtu1^Flox mice. The level of mitochondrial translation was markedly reduced in Mtu1-deficient hepatocytes compared with control cells (Fig 5A). Interestingly, the degree of impairment in 13 mitochondrial proteins depended on their molecular weights. The translation of 9 mitochondrial proteins with molecular weights higher than 25 kDa (equal to the molecular weight of COII/III) was markedly impaired in Mtu1-deficient cells (Fig 5A). On the other hand, the translation of the remaining 4 mitochondrial proteins (ND6, ND3, ND4L and A8) with molecular weights lower than 25 kDa was only slightly increased in Mtu1-deficient cells (Fig 5A).

Download:

Fig 5. Mtu1 deficiency impaired mitochondrial translation and respiratory activities in hepatocytes.

(A) Autoradiogram of mitochondrial translation in primary hepatocytes isolated from control (Flox) and hepatocyte-specific Mtu1 knockout (LKO) mice. (B) Protein levels of representative mitochondrial proteins were examined by western blotting. CI~CV indicates Complexes I ~ V. (C) Representative blue-native gel image of respiratory complexes purified from Flox and LKO mice. (D) Mitochondrial proteins incorporated in Complexes I ~ V were examined by blue-native PAGE followed by western blotting. (E) The activities of Complexes I ~ IV in the livers of Flox and LKO mice are shown. Individual complex activity was normalized to the activity of citrate synthase (CS). n = 3 each. **P < 0.01, ***P < 0.001.

https://doi.org/10.1371/journal.pgen.1006355.g005

The impairment in mitochondrial translation resulted in a decrease in the steady-state level of mitochondrial proteins (Fig 5B). Notably, the protein levels of NDUFB8 and MTCOI, which comprise Complexes I and IV, respectively, showed a marked reduction in the livers of Mtu1^LKO mice (Fig 5B). Accordingly, the formation of respiratory Complexes I~IV was impaired in Mtu1^LKO mice (Fig 5C and 5D). The disruption of mitochondrial translation consequently resulted in a broad and significant decrease in the activities of Complexes I, III and IV (Complex I: 70%, Complex III: 67%, Complex IV: 52% versus Flox mice, Fig 5E). There was also a significant increase of citrate synthase activity in the livers of Mtu1^LKO mice. These results clearly demonstrate that Mtu1 is indispensable for mitochondrial translation and respiratory activities.

Aberrant mitochondrial morphology in Mtu1-deficient hepatocytes

Because mitochondrial dynamics are closely coupled with mitochondrial proteostasis [23], we examined mitochondrial morphology using electron microscopy. Striking mitochondrial enlargement and proliferation were observed in Mtu1-deficient hepatocytes (Fig 6A). The average mitochondrial area in Mtu1-deficient hepatocytes was 4.3-fold larger than that in control hepatocytes (Fig 6B). Notably, nearly all mitochondria in Mtu1-deficient hepatocytes exhibited aberrant cristae structures. The cristae were either abnormally swollen or lost in most of the mitochondria (Fig 6C). Some mitochondria contained an inner vacuole with multiple layers of membrane, and some exhibited very low electron density (Fig 6C). Disruption of mitochondrial function has been associated with the activation of the pathway related to mitochondrial proteostasis [24]. In agreement with the previous findings, there was a substantial increase in proteins related to proteostasis, such as LONP1, AFG3L2, DRP1, MFN1 and PARKIN (Fig 6D). Taken together, these results demonstrate that Mtu1-mediated mitochondrial translation is required for the maintenance of mitochondrial structures and proteostasis.

Download:

Fig 6. Aberrant mitochondrial morphology in Mtu1-deficient hepatocytes.

(A) Representative electron microscopy images of hepatocytes in control (Flox) and hepatocyte-specific Mtu1 knockout (LKO) mice. Bar = 5 μm. (B) The mitochondrial area in Flox and LKO hepatocytes was examined by histogram and scatter plot (Insert). n = 300 and 330 for Flox and LKO, respectively. ***P < 0.001. (C) Representative images of hepatic mitochondria at high magnification. Bar = 1 μm. Boxes with dashed and solid lines indicate aberrant structures magnified in lower panels. (D) Examination of the amounts of proteins related to mitochondrial proteostasis by western blotting. Total mitochondrial proteins were stained and used as a loading control. Arrow indicates bands corresponding to AFG3L2.

https://doi.org/10.1371/journal.pgen.1006355.g006

Activation of compensatory signaling in Mtu1-deficient hepatocytes

The Mtu1^LKO mice showed severe mitochondrial dysfunction in hepatocytes but maintained liver function. We investigated the molecular mechanism that enables Mtu1^LKO mice to tolerate severe mitochondrial dysfunction in hepatocytes. Mitochondrial dysfunction often induces an increase in hepatic Fgf21 levels, which has been associated with compensatory signaling, such as mitochondrial biogenesis [25, 26]. There was an approximately 32-fold increase in the Fgf21 levels in the livers of Mtu1^LKO mice (Fig 7A). Accordingly, peroxisome proliferator-activated receptor gamma coactivator 1-alpha (Pgc1α), an upstream regulator of mitochondrial proliferation, was significantly up-regulated (Fig 7A). Accordingly, there was an approximately 3-fold increase of the mtDNA copy number, which was associated with an approximately 4-fold increase in the mtDNA-encoded mitochondrial genes in Mtu1-deficient hepatocytes (Fig 7B–7C). In addition, MTOR and ERK1/2, which are effectors of FGF21 [27–28], were also up-regulated at both the total protein level and phosphorylation level in Mtu1-deficient primary hepatocytes (Fig 7D).

Download:

Fig 7. Enhancement of mitochondrial biogenesis and oxidative stress response in Mtu1-deficient hepatocytes.

(A) Relative expression of Pgc1α and Fgf21 in the livers of control (Flox) and knockout (LKO) mice. n = 4 each. **P < 0.01. (B) The ratios of mitochondrial DNA (mtDNA) levels to nuclear DNA (nDNA) levels in the livers of Flox and LKO mice are shown. n = 4 each. ***P < 0.001. (C) Relative expression of mitochondrial DNA-encoded mitochondrial genes in the livers of Flox and LKO mice. n = 4 each. *P < 0.05, **P < 0.01. (D) Western blotting revealing an increase in MTOR, phospho-MTOR (p-MTOR), ERK1/2 and phospho-ERK1/2 levels in primary hepatocytes. (E) Examination of protein carbonylation by Oxyblot in mitochondria isolated from Flox and LKO livers. Total mitochondrial proteins were stained with CBB and used as a loading control. Asterisks indicate negative control samples. (F) Expression levels of genes related to the oxidative stress response were examined by quantitative PCR (n = 4 each). The relative expression levels are shown in a heat map. *P <0.05, **P < 0.01, ***P < 0.001.

https://doi.org/10.1371/journal.pgen.1006355.g007

Mitochondria are the major source for the production of reactive oxygen species, and its dysfunction has been associated with oxidative stress [29]. We examined how oxidative stress was managed in Mtu1-deficient hepatocytes. Surprisingly, there was a decrease in mitochondrial protein carbonylation, which is a byproduct of oxidative stress, in the livers of Mtu1^LKO mice (Fig 7E). In addition, we examined the levels of oxidative stress-related metabolites in the liver tissues (S4 Fig). The glutathione (GSH) and cysteine levels in Mtu1^LKO mice did not differ from those in Mtu1^Flox mice. Interestingly, the level of glutathione disulfide (GSSG), a marker of oxidative stress, trended toward a decrease in the livers of Mtu1^LKO mice (S4 Fig). These results prompted us to examine the gene profiles that are related to oxidative stress in liver tissues. These genes were dynamically changed in the livers of Mtu1^LKO mice, indicating an active response to oxidative stress in the Mtu1^LKO mice (Fig 7F). Importantly, antioxidant genes, such as glutathione synthetase (Gss), glutathione peroxidase (Gpx2/3) and sulfiredoxin 1 (Srxn1), were significantly up-regulated. Together, these results show that the increase in mitochondrial biogenesis in combination with the adaptive scavenging of oxidative stress might compensate for the mitochondrial dysfunction and prevent catastrophic liver failure in Mtu1^LKO mice.

Sustained liver function and compensatory signaling in adult Mtu1^LKO mice

Finally, to evaluate the progression of liver injury in Mtu1^LKO mice, we examined the histological, biochemical and genetic features of the livers at 16 weeks. The Mtu1^LKO mice were alive and exhibited sustained liver function. Serum ALT and AST levels in 16-week-old Mtu1^LKO mice, which were at the same levels as those of 3-week-old Mtu1^LKO mice, were still higher than the levels in 16-week-old Mtu1^Flox mice (Fig 8A). Unlike the 3-week-old mice, the serum LDH levels in the 16-week-old Mtu1^LKO mice did not differ from those of the Mtu1^Flox mice (Fig 8A). Similar to the histological features of 3-week-old mice, 16-week-old Mtu1^LKO mice also exhibited enlarged hepatocytes with karyomegaly and spotty necrosis; however, no obvious fibrosis was observed (Fig 8B).

Download:

Fig 8. Sustained liver function in adult Mtu1-deficient mice.

(A) Serum AST, ALT and LDH levels in LKO and Flox mice at the age of 16 weeks. n = 3 per genotype, **P < 0.01. (B) H&E and Azan staining in 16-week-old LKO and Flox mice. The arrow indicates spotty necrosis. Arrowheads indicate enlarged hepatocytes with karyomegaly. Bar = 0.2 mm for H&E staining. Bar = 0.1 mm for Azan staining. (C) Protein levels of representative mitochondrial proteins in the livers of 16-week-old Flox and LKO mice were examined by western blotting. (D) Mitochondrial proteins incorporated in Complexes I ~ V were examined by blue-native PAGE followed by western blotting. (E) The relative expression levels of Fgf21, Pgc1a, Gpx3 and Srxn1 in the livers of Flox and LKO mice are shown. n = 3 each. *P < 0.05, **P < 0.01, ****P < 0.0001. (F) The ratios of mtDNA levels to ntDNA levels in the livers of 16-week-old Flox and LKO mice are shown. n = 3 each. **P < 0.01.

https://doi.org/10.1371/journal.pgen.1006355.g008

Biochemical examination of mtDNA-derived MTCOI in total tissue lysates and in purified respiratory complexes revealed that the protein levels of MTCOI remained at low levels in 16-week-old Mtu1^LKO mice (Fig 8C–8D). Nevertheless, it is worthwhile to indicate that MTCOI levels appeared to be slightly increased compared to 3-week-old Mtu1^LKO mice (Fig 5D). At the gene expression level, Mtu1^LKO mice exhibited a marked up-regulation of Fgf21 at 16 weeks (Fig 8E). Genes related to mitochondrial proliferation and suppression of oxidative stress, such as Pgc1a, Gpx3 and Srxn1, also remained up-regulated in Mtu1^LKO mice compared to age-matched Mtu1^flox mice (Fig 8E). Accordingly, the relative mt-DNA copy number was up-regulated in 16-week-old Mtu1^LKO mice (Fig 8F). Taken together, these results suggest that despite the lasting mitochondrial dysfunction from embryo to adulthood, Mtu1^LKO mice were able to adapt to the liver injury and even exhibited some features of recovery in adulthood.

Discussion

In the present study, we established hepatocyte-specific Mtu1-deficient mice that manifest the clinical symptoms of RILF. Mtu1 deficiency in hepatocytes resulted in a marked reduction in mitochondrial translation. The impairment in mitochondrial translation subsequently caused a broad decrease in respiratory activities and led to the disruption of membrane integrity. The mitochondrial dysfunction consequently induced liver injury. Our murine model provides mechanistic insights into the pathogenesis of RILF.

Mutations in TRMU (MTU1) have been implicated in the pathogenesis of RILF [20]. To date, 20 RILF patients carrying pathogenic mutations in the coding region of MTU1 have been reported [20]. In contrast to the genetic evidence, the mechanism of RILF remains controversial. Some studies have reported that Mtu1 deficiency alone does not always cause the decrease in mitochondrial translation in RILF patient-derived cell lines [21–22]. In contrast, we showed that Mtu1 deficiency resulted in a marked impairment in mitochondrial translation and respiration in yeast and human cancer cell lines [19]. This discrepancy was likely caused by different experimental conditions in these studies. Indeed, all these studies were performed in cells that originated from different species. Notably, none of the previous studies were performed in cells related to the liver, which is the symptomatic tissue in RILF. In the present study, we generated liver-specific Mtu1 knockout mice, which allow us to investigate the role of Mtu1 in hepatocytes for the first time. Consistent with our previous results, Mtu1 deficiency markedly inhibited mitochondrial translation in hepatocytes, resulting in a substantial decrease in respiratory complexes and activities. Thus, our results lead to a clear conclusion that Mtu1 is required for mitochondrial translation in hepatocytes.

Why is Mtu1-mediated s² modification crucial for mitochondrial translation? A previous study showed that bacterial tRNA^Gln lacking the s² modification was still capable of translating the GAA codon, but the decoding efficiency of s²-deficient tRNA^Gln was 4-fold lower than that of a fully modified tRNA^Gln [30]. Therefore, it is conceivable that the major role of the s² modification at 34U is to facilitate base-pairing with A to increase decoding efficiency. In mice and humans, mitochondrial genes predominantly utilize the GAA, CAA and AAA codons, which are decoded by mt-tRNA^Glu, mt-tRNA^Gln and mt-tRNA^Lys, respectively (S5 Fig). It is likely that mitochondria perverted the s² modification during evolution for the optimal translation of biased codons. In addition, the codon usage might also influence the translation efficiency. In fact, the abundance of GAA, CAA and AAA codons is proportional to the length of mRNA, whereas the frequency of these codons did not differ among the mitochondrial genes (S5 Fig). Therefore, s² modification would be particularly required for the efficient translation of long mRNAs because of their high demand for their corresponding tRNAs.

Despite the important role of s² modification in regulating efficient translation, the s² modification level only ranges from 40%~70% at steady state. It is likely that GAA, CAA and AAA codons would be preferentially and efficiently decoded by fully modified mt-tRNAs in wild-type mitochondria. However, the unmodified mt-tRNAs might still be partially functional because mitochondrial translation was still detectable in Mtu1-deficient cells. Supporting this speculation, a complete loss of the mcm⁵s² modification, the cytosolic counterpart of τm⁵s², in a subset of yeast cytosolic tRNAs resulted in a lethal phenotype that was rescued by overexpressing unmodified tRNA^Lys(UUU) [31].

The Mtu1^LKO mice showed hepatic inflammation, necrosis, and elevated plasma levels of lactate and AST. These pathological features closely mimic the clinical symptoms of RILF [20]. However, compared with RILF patients, the phenotypes of Mtu1^LKO mice were rather moderate. Notably, the Mtu1^LKO mice did not exhibit hepatic fibrosis and nodule formation, which are frequently observed in RILF patients [20]. The genetic background of the Mtu1^LKO mice might explain the mild hepatic injury. There is substantial evidence to suggest that mice with the C57BL6 background are resistant to hepatic fibrosis [32–33]. Despite this resistance, the Mtu1^LKO mice still exhibited symptoms of liver injury, which further emphasizes the critical role of Mtu1-mediated mitochondrial translation in the development of RILF.

While the hepatocyte-specific Mtu1 knockout mice were viable, the constitutive knockout mice were embryonic lethal at a very early developmental stage. In agreement with our results, the constitutive deficiency of murine Dars2 (mitochondrial aspartyl-tRNA synthetase), which is a component of the mitochondrial translation machinery, is also embryonic lethal at a very early developmental stage [26]. These results suggest that efficient mitochondrial translation is indispensable for embryonic development. Importantly, lethality due to Mtu1 deficiency has been observed in RILF patients. Indeed, 6 of 20 patients died of acute liver failure between 1 and 8 months of age [20]. Three of the 6 patients carried homozygous mutations in either the translational start codon (Met1Lys) or the active site (Asn96Ser). These mutations are predicted to cause a complete loss of Mtu1 or its enzymatic activity in the patients. In contrast, many of the surviving patients carried mutations in non-essential domains, which presumably cause a partial inhibition of Mtu1 activity. Taken together, these results suggest that the clinical progression of RILF might depend on the level of remaining Mtu1 activity in the tissues.

Mtu1-mediated s² modification requires a complicated enzymatic reaction that transfers the sulfur atom from cysteine to tRNAs [34]. Because cysteine metabolism is limited during neonatal development, it is proposed that cysteine availability might contribute to the development of liver failure in patients carrying pathogenic mutations [11, 21] However, the cysteine levels in liver tissues of Mtu1^LKO mice did not differ from those of Mtu1^Flox mice. In addition, sulfur-containing tRNA modifications, including cytosolic mcm⁵s²U modifications and mitochondrial ms²i⁶A modifications, remained intact in Mtu1-deficient cells. Our results suggest that cysteine availability is likely not involved in the pathological phenotypes in our mouse model.

The reversibility is the most interesting feature of RILF. After surviving the acute phase, the patients spontaneously recover without recurrence due to unknown mechanisms [20]. Mitochondrial biogenesis is a potential compensatory effect for mitochondrial dysfunction [26]. Indeed, we observed marked mitochondrial biogenesis in response to Mtu1 deficiency. Mitochondrial biogenesis is most likely activated by up-regulation of Pgc1α signaling. This result was consistent with the observation in Dars2 knockout mice, which also showed up-regulation of Pgc1α expression and mitochondrial biogenesis [26]. In addition to the mitochondrial effect, our study revealed a unique compensatory effect involving suppression of oxidative stress. Although mitochondrial dysfunction is usually associated with the generation of oxidative stress [29], there was a moderate reduction in the stress levels and a marked increase in antioxidant gene expression in Mtu1-deficient hepatocytes. It is likely that the Mtu1 deficiency triggers oxidative stress due to severe mitochondrial dysfunction, but the adaptive scavenging response is strong enough to suppress the stress to a rather low level. Intriguingly, up-regulation of antioxidant genes in Mtu1^LKO mice has been observed from the adolescent stage to the adult stage. The continuous activation of mitochondrial biogenesis and the suppression of oxidative stress might protect Mtu1^LKO mice from catastrophic liver failure and maintain liver function in a tolerable condition from embryo to adulthood. From this perspective, treating RIFL patients with either cysteine or N-acetylcysteine might suppress oxidative stress and assist an early recovery.

In addition to RILF, the Mtu1-mediated s² modification has also been implicated in reversible infantile respiratory chain deficiency (RIRCD) [20]. RIRCD patients exhibit severe myopathy in the first months of life, followed by spontaneous recovery with some mild residual myopathy. The molecular mechanism underlying RIRCD is unknown; however, genetic analysis has revealed a single homoplasmic m.14674T>C mutation in mitochondrial DNA that corresponds to mt-tRNA^Glu [35–37]. Interestingly, there was a decrease in the s² modification in mt-tRNA^Glu in muscle samples with an m.14674T>C mutation [21]. Similar to RILF, Boczonadi et al. reported that the decrease in s² modification was not associated with the impairment of mitochondrial translation in fibroblasts and myoblast cells established from RIRCD patients [21]. Given the different regulatory mechanisms in immortal cells and intact tissues, it is likely that the m.14674T>C mutation might also affect mitochondrial translation in the tissues of RIRCD patients. Further study using muscle-specific Mtu1-deificient mice may shed light on the molecular mechanism of RIRCD.

In summary, we demonstrated that Mtu1-mediated s² modification of mt-tRNA is indispensable for efficient mitochondrial translation and activities. Our study suggests that mitochondrial dysfunction due to Mtu1 deficiency is the primary cause of RILF. Our murine model is a valuable tool for understanding the molecular mechanism of RILF and for developing effective treatments.

Materials and Methods

Animals

Constitutive Mtu1 knockout mice were generated by crossing transgenic mice harboring exon 2 of the Mtu1 gene floxed by LoxP sequences (Mtu1^f/f mice) with transgenic mice expressing Cre recombinase under the control of the CAG promoter (CAGCre mice). Liver-specific Mtu1 KO mice were generated by crossing Mtu1^f/f mice with transgenic mice carrying Cre recombinase under the control of the albumin promoter (AlbCre mice). Mtu1^f/f mice, CAGCre transgenic mice and AlbCre transgenic mice were backcrossed with C57BL6/J mice for at least seven generations to control the genetic background. Mice were housed at 25°C with 12 h light and 12 h dark cycles. Unless otherwise indicated, we sacrificed 3- to 5-week-old male mice for all experiments in Figs 1–7. All animal procedures were approved by the Animal Ethics Committee of Kumamoto University (Approval ID: A27-037). Detailed information on genotyping can be found in the “Supplemental Methods”.

Primary hepatocyte culture

Primary hepatocytes were isolated from Mtu1^f/f and Mtu1^LKO mice by perfusion of collagenase (Worthington Biochemical Corporation, Lakewood, NJ) following the manufacturer’s instructions. Isolated hepatocytes were cultured in high glucose DMEM (Thermo Fisher Scientific, Waltham, MA) supplemented with 10% fetal bovine serum (Hyclone, GE Healthcare, NJ) for 3 h. Subsequently, the culture medium was replaced with DMEM without serum for 14 h. All experiments using primary hepatocytes were performed within 24 h after isolation.

Gene expression analysis

Total RNA was isolated from fresh liver samples using TRIzol reagent (ThermoFisher Scientific, USA) following the manufacturer’s instructions. cDNA was synthesized from 100 ng of total RNA using the PrimerScript RT-PCR kit (TAKARA, Tokyo, Japan) and subjected to quantitative PCR (SYBR Premix Ex Taq II, TAKARA) using a 7300 Real Time PCR System (Thermo Fisher Scientific, CA). The sequence information is included in the Supplemental Methods.

Western blotting

The mitochondrial fraction was isolated from the livers of conditional Mtu1 knockout mice or HeLa cells using MOPS buffer as described previously. Ten micrograms of each sample were loaded into 12% SDS-PAGE gels and transferred to PVDF membranes. Mitochondrial and cellular proteins were detected using the proper antibodies as described in the supporting information.

Statistics

The data were analyzed using GraphPad Prism 6 software. An unpaired Student’s t-test was used to test the differences between two groups. A 2-tailed P-value of 0.05 was considered significant. The results are shown as the means ± S.E.M.

Detail methods are provided in the “Supporting Information”.

Supporting Information

S1 Fig. Morphological examination of liver-specific Mtu1 knockout mice.

(A) Strategy for the generation of liver-specific Mtu1 knockout mice (Mtu1^LKO: LKO). Mice carrying the floxed Mtu1 gene were used as a control (Mtu1^Flox: Flox). (B) Representative male Mtu1^LKO and Mtu1^Flox mice at 6 weeks of age. (C) Representative genotyping results of the Mtu1^LKO and Mtu1^Flox mice shown in (B). (D) Representative H&E staining of liver sections of control mice (Flox) and Mtu1^LKO mice (LKO). Bars = 0.2 mm.

https://doi.org/10.1371/journal.pgen.1006355.s001

(TIF)

S2 Fig. Relative amount of modifications at 34U.

(A-C) Individual mt-tRNA^Lys, mt-tRNA^Glu and mt-tRNA^Gln were isolated from Mtu1^Flox and Mtu1^LKO mice and subjected to mass spectrometry analysis. Representative mass chromatograms of mt-tRNA fragments containing τm⁵U, τm⁵s²U, s²U or U at position 34 were shown. Arrowheads indicate traces of fragments containing s² modification in LKO mice. (D) The relative amounts of τm⁵U, τm⁵s²U, s²U and U at position 34 were calculated from the peak areas and plotted.

https://doi.org/10.1371/journal.pgen.1006355.s002

(TIF)

S3 Fig. Sulfur-containing tRNA modifications in Mtu1^LKO mice.

Total RNA was isolated from the livers of 3-week-old Mtu1^LKO and Mtu1^Flox mice. RNA was digested and subjected to mass spectrometry. The levels of mcm⁵s²U and ms²i⁶A modifications were normalized to the levels of mcm⁵U and i⁶A modifications, respectively. n = 4 each.

https://doi.org/10.1371/journal.pgen.1006355.s003

(TIF)

S4 Fig. Glutathione and glutathione disulfide levels in Mtu1^LKO mice.

(A) Relative levels of glutathione disulfide (GSSG) in liver tissues of 3-week-old Mtu1^LKO and Mtu1^flox mice (LKO: 61% versus Flox mice). n = 4; P = 0.059. (B) Relative levels of glutathione (GSH) (LKO: 117% versus Flox mice). n = 4; P = 0.4. (C) Relative GSSG/GSH ratios (LKO: 50% versus Flox mice). n = 4; P = 0.057. (D) Relative levels of cysteine (LKO: 92% versus Flox mice). n = 4; P = 0.71.

https://doi.org/10.1371/journal.pgen.1006355.s004

(TIF)

S5 Fig. Codon usage in mouse and human mitochondrial genes.

(A) Codon numbers of Lys (AAA, AAG), Glu (GAA, GAG) and Gln (CAA, CAG) in mouse and human mitochondrial mRNAs. Yellow columns represent the 4 transcripts that exhibited normal translation in Mtu1-deficient hepatocytes. (B) Codon frequencies of AAA/GAA/CAA and AAG/GAG/CAG in mouse and human mitochondrial mRNAs. The 4 transcripts shown in yellow letters correspond to the 4 transcripts that exhibited normal translation in Mtu1-deficient hepatocytes. (C) Correlation of the number of AAA/GAA/CAA codons with the total length of the transcripts. P = 0.001.

https://doi.org/10.1371/journal.pgen.1006355.s005

(TIF)

S1 Text. Supplemental Methods.

https://doi.org/10.1371/journal.pgen.1006355.s006

(DOCX)

Acknowledgments

We thank Ms. Nobuko Maeda for technical assistance.

Author Contributions

Conceptualization: TsS FYW KT.
Funding acquisition: FYW KT.
Investigation: YW LK TaS KA AF TK YO YK MT.
Supervision: FYW KT.
Writing – original draft: YW FYW.
Writing – review & editing: FYW KT.

References

1. Agris PF. Decoding the genome: a modified view. Nucleic Acids Res 2004;32: 223–238. pmid:14715921
- View Article
- PubMed/NCBI
- Google Scholar
2. Machnicka MA, Milanowska K, Osman Oglou O, Purta E, Kurkowska M, Olchowik A, et al. MODOMICS: a database of RNA modification pathways—2013 update. Nucleic Acids Res 2013;41(Database issue): D262–267. pmid:23118484
- View Article
- PubMed/NCBI
- Google Scholar
3. Suzuki T, Suzuki T. A complete landscape of post-transcriptional modifications in mammalian mitochondrial tRNAs. Nucleic Acids Res 2014;42: 7346–7357. pmid:24831542
- View Article
- PubMed/NCBI
- Google Scholar
4. Suzuki T. Biosynthesis and function of tRNA wobble modifications. Topics in Current Genetics 2005;12: 24–69.
- View Article
- Google Scholar
5. Suzuki T, Nagao A, and Suzuki T. Human mitochondrial tRNAs: Biogenesis, function, structural aspects and diseases. Annu Rev Genet 2011;45: 299–329. pmid:21910628
- View Article
- PubMed/NCBI
- Google Scholar
6. Kremer LS, L'hermitte-Stead C, Lesimple P, Gilleron M, Filaut S, Jardel C, et al. Severe respiratory complex III defect prevents liver adaptation to prolonged fasting. J Hepatol 2016;65: 377–385. pmid:27151179
- View Article
- PubMed/NCBI
- Google Scholar
7. Martín MÁ, García-Silva MT, Barcia G, Delmiro A, Rodríguez-García ME, Blázquez A, et al. The homozygous R504C mutation in MTO1 gene is responsible for ONCE syndrome. Clin Gene 2016; In Press.
- View Article
- Google Scholar
8. Charif M, Titah SM, Roubertie A, Desquiret-Dumas V, Gueguen N, Meunier I, et al. Optic neuropathy, cardiomyopathy, cognitive disability in patients with a homozygous mutation in the nuclear MTO1 and a mitochondrial MT-TF variant. Am J Med Genet A 2015;167A: 2366–2374. pmid:26061759
- View Article
- PubMed/NCBI
- Google Scholar
9. Kopajtich R, Nicholls TJ, Rorbach J, Metodiev MD, Freisinger P, Mandel H, et al. Mutations in GTPBP3 cause a mitochondrial translation defect associated with hypertrophic cardiomyopathy, lactic acidosis, and encephalopathy. Am J Hum Genet 2014;95: 708–720. pmid:25434004
- View Article
- PubMed/NCBI
- Google Scholar
10. Zeharia A, Shaag A, Pappo O, Mager-Heckel AM, Saada A, Beinat M, et al. Acuteinfantile liver failure due to mutations in the TRMU gene. Am J Hum Genet 2009;85: 401–407. pmid:19732863
- View Article
- PubMed/NCBI
- Google Scholar
11. Schara U, von Kleist-Retzow JC, Lainka E, Gerner P, Pyle A, Smith PM, et al. Acute liverfailure with subsequent cirrhosis as the primary manifestation of TRMU mutations. J Inherit Metab Dis 2011;34: 197–201. pmid:21153446
- View Article
- PubMed/NCBI
- Google Scholar
12. Uusimaa J, Jungbluth H, Fratter C, Crisponi G, Feng L, Zeviani M, et al. Reversible infantile respiratory chain deficiency is a unique, genetically heterogenous mitochondrial disease. J Med Genet 2011;48: 660–668. pmid:21931168
- View Article
- PubMed/NCBI
- Google Scholar
13. Gaignard P, Gonzales E, Ackermann O, Labrune P, Correia I, Therond P, et al. Mitochondrial Infantile Liver Disease due to TRMU Gene Mutations: Three New Cases. JIMD Rep 2013;11: 117–123. pmid:23625533
- View Article
- PubMed/NCBI
- Google Scholar
14. Zeharia A, Fischel-Ghodsian N, Casas K, Bykhocskaya Y, Tamari H, Lev D, et al. Mitochondrial myopathy, sideroblastic anemia, and lactic acidosis: an autosomal recessive syndrome in Persian Jews caused by a mutation in the PUS1 gene. J Child Neurol 2005;20: 449–452. pmid:15971356
- View Article
- PubMed/NCBI
- Google Scholar
15. Mangum JE, Hardee JP, Fix DK, Puppa MJ, Elkes J, Altomare D, et al. Pseudouridine synthase 1 deficient mice, a model for Mitochondrial Myopathy with Sideroblastic Anemia, exhibit muscle morphology and physiology alterations. Sci Rep 2016; 6:26202. pmid:27197761
- View Article
- PubMed/NCBI
- Google Scholar
16. Wei FY, Zhou B, Suzuki T, Miyata K, Ujihara Y, Horiguchi H, et al. Cdk5rap1-mediated 2-methylthio modification of mitochondrial tRNAs governs protein translation and contributes to myopathy in mice and humans. Cell Metab 2015;21: 428–442. pmid:25738458
- View Article
- PubMed/NCBI
- Google Scholar
17. Suzuki T, Suzuki T, Wada T, Saigo K, Watanabe K. Taurine as a constituent of tochondrial tRNAs: new insights into the functions of taurine and human mitochondrial diseases. EMBO J 2002;21: 6581–6589. pmid:12456664
- View Article
- PubMed/NCBI
- Google Scholar
18. Yasukawa T, Suzuki T, Ishii N, Ohta S, Watanabe K. Wobble modification defect in tRNA disturbs codon-anticodon interaction in a mitochondrial disease. EMBO J 2001;20: 4794–4802. pmid:11532943
- View Article
- PubMed/NCBI
- Google Scholar
19. Umeda N, Suzuki T, Yukawa M, Ohya Y, Shindo H, Watanabe K, et al. Mitochondria-specific RNA-modifying enzymes responsible for the biosynthesis of the wobble base in mitochondrial tRNAs. Implications for the molecular pathogenesis of human mitochondrial diseases. J Biol Chem 2005;280: 1613–1624. pmid:15509579
- View Article
- PubMed/NCBI
- Google Scholar
20. Boczonadi V, Bansagi B, Horvath R. Reversible infantile mitochondrial diseases. J Inherit Metab Dis 2015;38: 427–435. pmid:25407320
- View Article
- PubMed/NCBI
- Google Scholar
21. Boczonadi V, Smith PM, Pyle A, Gomez-Duran A, Schara U, Tulinius M, et al. Altered 2-thiouridylation impairs mitochondrial translation in reversible infantile respiratory chain deficiency. Hum Mol Genet 2013;22: 4602–4615. pmid:23814040
- View Article
- PubMed/NCBI
- Google Scholar
22. Sasarman F, Antonicka H, Horvath R, Shoubridge EA. The 2-thiouridylase function of the human MTU1 (TRMU) enzyme is dispensable for mitochondrial translation. Hum Mol Genet 2011;20: 4634–4643. pmid:21890497
- View Article
- PubMed/NCBI
- Google Scholar
23. Civiletto G, Varanita T, Cerutti R, Gorletta T, Barbaro S, Marchet S, et al. Opa1 overexpression ameliorates the phenotype of two mitochondrial disease mouse models. Cell Metab 2015;21: 845–854. pmid:26039449
- View Article
- PubMed/NCBI
- Google Scholar
24. Houtkooper RH, Mouchiroud L, Ryu D, Moullan N, Katsyuba E, Knott G, et al. Mitonuclear protein imbalance as a conserved longevity mechanism. Nature 2013;497: 451–457. pmid:23698443
- View Article
- PubMed/NCBI
- Google Scholar
25. Fisher FM, Maratos-Flier E. Understanding the Physiology of FGF21. Annu Rev Physiol 2016;78: 223–241. pmid:26654352
- View Article
- PubMed/NCBI
- Google Scholar
26. Dogan SA, Pujol C, Maiti P, Kukat A, Wang S, Hermans S, et al. Tissue-specific loss of DARS2 activates stress responses independently of respiratory chain deficiency in the heart. Cell Metab 2014;19: 458–469. pmid:24606902
- View Article
- PubMed/NCBI
- Google Scholar
27. Cornu M, Oppliger W, Albert V, Robitaille AM, Trapani F, Quagliata L, et al. Hepatic mTORC1 controls locomotor activity, body temperature, and lipid metabolism through FGF21. Proc Natl Acad Sci U S A 2014;111: 11592–11599. pmid:25082895
- View Article
- PubMed/NCBI
- Google Scholar
28. Wang X, Wei W, Krzeszinski JY, Wang Y, Wan Y. A Liver-Bone Endocrine Relay by IGFBP1 Promotes Osteoclastogenesis and Mediates FGF21-Induced Bone Resorption. Cell Metab 2015;22: 811–824. pmid:26456333
- View Article
- PubMed/NCBI
- Google Scholar
29. López-Otín C, Blasco MA, Partridge L, Serrano M, Kroemer G. The hallmarks of aging. Cell 2013;153: 1194–1217. pmid:23746838
- View Article
- PubMed/NCBI
- Google Scholar
30. Krüger MK, Pedersen S, Hagervall TG, Sørensen MA. The modification of the wobble base of tRNAGlu modulates the translation rate of glutamic acid codons in vivo. J Mol Biol 1998;284: 621–631. pmid:9826503
- View Article
- PubMed/NCBI
- Google Scholar
31. Björk GR, Huang B, Persson OP, Byström AS. A conserved modified wobble nucleoside (mcm5s2U) in lysyl-tRNA is required for viability in yeast. RNA 2007;13: 1245–1255. pmid:17592039
- View Article
- PubMed/NCBI
- Google Scholar
32. Walkin L, Herrick SE, Summers A, Brenchley PE, Hoff CM, Korstanje R, et al. The role of mouse strain differences in the susceptibility to fibrosis: a systematic review. Fibrogenesis Tissue Repair 2013;6: 18. pmid:24294831
- View Article
- PubMed/NCBI
- Google Scholar
33. Shi Z, Wakil AE, Rockey DC. Strain-specific differences in mouse hepatic wound healing are mediated by divergent T helper cytokine responses. Proc Natl Acad Sci U S A 1997;94: 10663–10668. pmid:9380692
- View Article
- PubMed/NCBI
- Google Scholar
34. Shigi N. Biosynthesis and functions of sulfur modifications in tRNA. Front Genet 2014;5: 67. pmid:24765101
- View Article
- PubMed/NCBI
- Google Scholar
35. Horvath R, Kemp JP, Tuppen HA, Hudson G, Oldfors A, Marie SK, et al. Molecular basis of infantile reversible cytochrome c oxidase deficiency myopathy. Brain 2009;132: 3165–3174. pmid:19720722
- View Article
- PubMed/NCBI
- Google Scholar
36. Mimaki M, Hatakeyama H, Komaki H, Yokoyama M, Arai H, Kirino Y, et al. Reversible infantile respiratory chain deficiency: a clinical and molecular study. Ann Neurol 2010;68: 845–854. pmid:21194154
- View Article
- PubMed/NCBI
- Google Scholar
37. Uusimaa J, Jungbluth H, Fratter C, Crisponi G, Feng L, Zeviani M, et al. Reversible infantile respiratory chain deficiency is a unique, genetically heterogenous mitochondrial disease. J Med Genet 2011;48: 660–668. pmid:21931168
- View Article
- PubMed/NCBI
- Google Scholar

[ref1] 1. Agris PF. Decoding the genome: a modified view. Nucleic Acids Res 2004;32: 223–238. pmid:14715921
View Article
PubMed/NCBI
Google Scholar

[2] View Article

[3] PubMed/NCBI

[4] Google Scholar

[ref2] 2. Machnicka MA, Milanowska K, Osman Oglou O, Purta E, Kurkowska M, Olchowik A, et al. MODOMICS: a database of RNA modification pathways—2013 update. Nucleic Acids Res 2013;41(Database issue): D262–267. pmid:23118484
View Article
PubMed/NCBI
Google Scholar

[6] View Article

[7] PubMed/NCBI

[8] Google Scholar

[ref3] 3. Suzuki T, Suzuki T. A complete landscape of post-transcriptional modifications in mammalian mitochondrial tRNAs. Nucleic Acids Res 2014;42: 7346–7357. pmid:24831542
View Article
PubMed/NCBI
Google Scholar

[10] View Article

[11] PubMed/NCBI

[12] Google Scholar

[ref4] 4. Suzuki T. Biosynthesis and function of tRNA wobble modifications. Topics in Current Genetics 2005;12: 24–69.
View Article
Google Scholar

[14] View Article

[15] Google Scholar

[ref5] 5. Suzuki T, Nagao A, and Suzuki T. Human mitochondrial tRNAs: Biogenesis, function, structural aspects and diseases. Annu Rev Genet 2011;45: 299–329. pmid:21910628
View Article
PubMed/NCBI
Google Scholar

[17] View Article

[18] PubMed/NCBI

[19] Google Scholar

[ref6] 6. Kremer LS, L'hermitte-Stead C, Lesimple P, Gilleron M, Filaut S, Jardel C, et al. Severe respiratory complex III defect prevents liver adaptation to prolonged fasting. J Hepatol 2016;65: 377–385. pmid:27151179
View Article
PubMed/NCBI
Google Scholar

[21] View Article

[22] PubMed/NCBI

[23] Google Scholar

[ref7] 7. Martín MÁ, García-Silva MT, Barcia G, Delmiro A, Rodríguez-García ME, Blázquez A, et al. The homozygous R504C mutation in MTO1 gene is responsible for ONCE syndrome. Clin Gene 2016; In Press.
View Article
Google Scholar

[25] View Article

[26] Google Scholar

[ref8] 8. Charif M, Titah SM, Roubertie A, Desquiret-Dumas V, Gueguen N, Meunier I, et al. Optic neuropathy, cardiomyopathy, cognitive disability in patients with a homozygous mutation in the nuclear MTO1 and a mitochondrial MT-TF variant. Am J Med Genet A 2015;167A: 2366–2374. pmid:26061759
View Article
PubMed/NCBI
Google Scholar

[28] View Article

[29] PubMed/NCBI

[30] Google Scholar

[ref9] 9. Kopajtich R, Nicholls TJ, Rorbach J, Metodiev MD, Freisinger P, Mandel H, et al. Mutations in GTPBP3 cause a mitochondrial translation defect associated with hypertrophic cardiomyopathy, lactic acidosis, and encephalopathy. Am J Hum Genet 2014;95: 708–720. pmid:25434004
View Article
PubMed/NCBI
Google Scholar

[32] View Article

[33] PubMed/NCBI

[34] Google Scholar

[ref10] 10. Zeharia A, Shaag A, Pappo O, Mager-Heckel AM, Saada A, Beinat M, et al. Acuteinfantile liver failure due to mutations in the TRMU gene. Am J Hum Genet 2009;85: 401–407. pmid:19732863
View Article
PubMed/NCBI
Google Scholar

[36] View Article

[37] PubMed/NCBI

[38] Google Scholar

[ref11] 11. Schara U, von Kleist-Retzow JC, Lainka E, Gerner P, Pyle A, Smith PM, et al. Acute liverfailure with subsequent cirrhosis as the primary manifestation of TRMU mutations. J Inherit Metab Dis 2011;34: 197–201. pmid:21153446
View Article
PubMed/NCBI
Google Scholar

[40] View Article

[41] PubMed/NCBI

[42] Google Scholar

[ref12] 12. Uusimaa J, Jungbluth H, Fratter C, Crisponi G, Feng L, Zeviani M, et al. Reversible infantile respiratory chain deficiency is a unique, genetically heterogenous mitochondrial disease. J Med Genet 2011;48: 660–668. pmid:21931168
View Article
PubMed/NCBI
Google Scholar

[44] View Article

[45] PubMed/NCBI

[46] Google Scholar

[ref13] 13. Gaignard P, Gonzales E, Ackermann O, Labrune P, Correia I, Therond P, et al. Mitochondrial Infantile Liver Disease due to TRMU Gene Mutations: Three New Cases. JIMD Rep 2013;11: 117–123. pmid:23625533
View Article
PubMed/NCBI
Google Scholar

[48] View Article

[49] PubMed/NCBI

[50] Google Scholar

[ref14] 14. Zeharia A, Fischel-Ghodsian N, Casas K, Bykhocskaya Y, Tamari H, Lev D, et al. Mitochondrial myopathy, sideroblastic anemia, and lactic acidosis: an autosomal recessive syndrome in Persian Jews caused by a mutation in the PUS1 gene. J Child Neurol 2005;20: 449–452. pmid:15971356
View Article
PubMed/NCBI
Google Scholar

[52] View Article

[53] PubMed/NCBI

[54] Google Scholar

[ref15] 15. Mangum JE, Hardee JP, Fix DK, Puppa MJ, Elkes J, Altomare D, et al. Pseudouridine synthase 1 deficient mice, a model for Mitochondrial Myopathy with Sideroblastic Anemia, exhibit muscle morphology and physiology alterations. Sci Rep 2016; 6:26202. pmid:27197761
View Article
PubMed/NCBI
Google Scholar

[56] View Article

[57] PubMed/NCBI

[58] Google Scholar

[ref16] 16. Wei FY, Zhou B, Suzuki T, Miyata K, Ujihara Y, Horiguchi H, et al. Cdk5rap1-mediated 2-methylthio modification of mitochondrial tRNAs governs protein translation and contributes to myopathy in mice and humans. Cell Metab 2015;21: 428–442. pmid:25738458
View Article
PubMed/NCBI
Google Scholar

[60] View Article

[61] PubMed/NCBI

[62] Google Scholar

[ref17] 17. Suzuki T, Suzuki T, Wada T, Saigo K, Watanabe K. Taurine as a constituent of tochondrial tRNAs: new insights into the functions of taurine and human mitochondrial diseases. EMBO J 2002;21: 6581–6589. pmid:12456664
View Article
PubMed/NCBI
Google Scholar

[64] View Article

[65] PubMed/NCBI

[66] Google Scholar

[ref18] 18. Yasukawa T, Suzuki T, Ishii N, Ohta S, Watanabe K. Wobble modification defect in tRNA disturbs codon-anticodon interaction in a mitochondrial disease. EMBO J 2001;20: 4794–4802. pmid:11532943
View Article
PubMed/NCBI
Google Scholar

[68] View Article

[69] PubMed/NCBI

[70] Google Scholar

[ref19] 19. Umeda N, Suzuki T, Yukawa M, Ohya Y, Shindo H, Watanabe K, et al. Mitochondria-specific RNA-modifying enzymes responsible for the biosynthesis of the wobble base in mitochondrial tRNAs. Implications for the molecular pathogenesis of human mitochondrial diseases. J Biol Chem 2005;280: 1613–1624. pmid:15509579
View Article
PubMed/NCBI
Google Scholar

[72] View Article

[73] PubMed/NCBI

[74] Google Scholar

[ref20] 20. Boczonadi V, Bansagi B, Horvath R. Reversible infantile mitochondrial diseases. J Inherit Metab Dis 2015;38: 427–435. pmid:25407320
View Article
PubMed/NCBI
Google Scholar

[76] View Article

[77] PubMed/NCBI

[78] Google Scholar

[ref21] 21. Boczonadi V, Smith PM, Pyle A, Gomez-Duran A, Schara U, Tulinius M, et al. Altered 2-thiouridylation impairs mitochondrial translation in reversible infantile respiratory chain deficiency. Hum Mol Genet 2013;22: 4602–4615. pmid:23814040
View Article
PubMed/NCBI
Google Scholar

[80] View Article

[81] PubMed/NCBI

[82] Google Scholar

[ref22] 22. Sasarman F, Antonicka H, Horvath R, Shoubridge EA. The 2-thiouridylase function of the human MTU1 (TRMU) enzyme is dispensable for mitochondrial translation. Hum Mol Genet 2011;20: 4634–4643. pmid:21890497
View Article
PubMed/NCBI
Google Scholar

[84] View Article

[85] PubMed/NCBI

[86] Google Scholar

[ref23] 23. Civiletto G, Varanita T, Cerutti R, Gorletta T, Barbaro S, Marchet S, et al. Opa1 overexpression ameliorates the phenotype of two mitochondrial disease mouse models. Cell Metab 2015;21: 845–854. pmid:26039449
View Article
PubMed/NCBI
Google Scholar

[88] View Article

[89] PubMed/NCBI

[90] Google Scholar

[ref24] 24. Houtkooper RH, Mouchiroud L, Ryu D, Moullan N, Katsyuba E, Knott G, et al. Mitonuclear protein imbalance as a conserved longevity mechanism. Nature 2013;497: 451–457. pmid:23698443
View Article
PubMed/NCBI
Google Scholar

[92] View Article

[93] PubMed/NCBI

[94] Google Scholar

[ref25] 25. Fisher FM, Maratos-Flier E. Understanding the Physiology of FGF21. Annu Rev Physiol 2016;78: 223–241. pmid:26654352
View Article
PubMed/NCBI
Google Scholar

[96] View Article

[97] PubMed/NCBI

[98] Google Scholar

[ref26] 26. Dogan SA, Pujol C, Maiti P, Kukat A, Wang S, Hermans S, et al. Tissue-specific loss of DARS2 activates stress responses independently of respiratory chain deficiency in the heart. Cell Metab 2014;19: 458–469. pmid:24606902
View Article
PubMed/NCBI
Google Scholar

[100] View Article

[101] PubMed/NCBI

[102] Google Scholar

[ref27] 27. Cornu M, Oppliger W, Albert V, Robitaille AM, Trapani F, Quagliata L, et al. Hepatic mTORC1 controls locomotor activity, body temperature, and lipid metabolism through FGF21. Proc Natl Acad Sci U S A 2014;111: 11592–11599. pmid:25082895
View Article
PubMed/NCBI
Google Scholar

[104] View Article

[105] PubMed/NCBI

[106] Google Scholar

[ref28] 28. Wang X, Wei W, Krzeszinski JY, Wang Y, Wan Y. A Liver-Bone Endocrine Relay by IGFBP1 Promotes Osteoclastogenesis and Mediates FGF21-Induced Bone Resorption. Cell Metab 2015;22: 811–824. pmid:26456333
View Article
PubMed/NCBI
Google Scholar

[108] View Article

[109] PubMed/NCBI

[110] Google Scholar

[ref29] 29. López-Otín C, Blasco MA, Partridge L, Serrano M, Kroemer G. The hallmarks of aging. Cell 2013;153: 1194–1217. pmid:23746838
View Article
PubMed/NCBI
Google Scholar

[112] View Article

[113] PubMed/NCBI

[114] Google Scholar

[ref30] 30. Krüger MK, Pedersen S, Hagervall TG, Sørensen MA. The modification of the wobble base of tRNAGlu modulates the translation rate of glutamic acid codons in vivo. J Mol Biol 1998;284: 621–631. pmid:9826503
View Article
PubMed/NCBI
Google Scholar

[116] View Article

[117] PubMed/NCBI

[118] Google Scholar

[ref31] 31. Björk GR, Huang B, Persson OP, Byström AS. A conserved modified wobble nucleoside (mcm5s2U) in lysyl-tRNA is required for viability in yeast. RNA 2007;13: 1245–1255. pmid:17592039
View Article
PubMed/NCBI
Google Scholar

[120] View Article

[121] PubMed/NCBI

[122] Google Scholar

[ref32] 32. Walkin L, Herrick SE, Summers A, Brenchley PE, Hoff CM, Korstanje R, et al. The role of mouse strain differences in the susceptibility to fibrosis: a systematic review. Fibrogenesis Tissue Repair 2013;6: 18. pmid:24294831
View Article
PubMed/NCBI
Google Scholar

[124] View Article

[125] PubMed/NCBI

[126] Google Scholar

[ref33] 33. Shi Z, Wakil AE, Rockey DC. Strain-specific differences in mouse hepatic wound healing are mediated by divergent T helper cytokine responses. Proc Natl Acad Sci U S A 1997;94: 10663–10668. pmid:9380692
View Article
PubMed/NCBI
Google Scholar

[128] View Article

[129] PubMed/NCBI

[130] Google Scholar

[ref34] 34. Shigi N. Biosynthesis and functions of sulfur modifications in tRNA. Front Genet 2014;5: 67. pmid:24765101
View Article
PubMed/NCBI
Google Scholar

[132] View Article

[133] PubMed/NCBI

[134] Google Scholar

[ref35] 35. Horvath R, Kemp JP, Tuppen HA, Hudson G, Oldfors A, Marie SK, et al. Molecular basis of infantile reversible cytochrome c oxidase deficiency myopathy. Brain 2009;132: 3165–3174. pmid:19720722
View Article
PubMed/NCBI
Google Scholar

[136] View Article

[137] PubMed/NCBI

[138] Google Scholar

[ref36] 36. Mimaki M, Hatakeyama H, Komaki H, Yokoyama M, Arai H, Kirino Y, et al. Reversible infantile respiratory chain deficiency: a clinical and molecular study. Ann Neurol 2010;68: 845–854. pmid:21194154
View Article
PubMed/NCBI
Google Scholar

[140] View Article

[141] PubMed/NCBI

[142] Google Scholar

[ref37] 37. Uusimaa J, Jungbluth H, Fratter C, Crisponi G, Feng L, Zeviani M, et al. Reversible infantile respiratory chain deficiency is a unique, genetically heterogenous mitochondrial disease. J Med Genet 2011;48: 660–668. pmid:21931168
View Article
PubMed/NCBI
Google Scholar

[144] View Article

[145] PubMed/NCBI

[146] Google Scholar

Figures

Abstract

Author Summary

Introduction

Results

Mtu1 is indispensable for embryonic development

Liver-specific Mtu1 knockout mice exhibited liver injury and altered metabolism

Mtu1-mediated s2 modification is essential for mitochondrial translation

Aberrant mitochondrial morphology in Mtu1-deficient hepatocytes

Activation of compensatory signaling in Mtu1-deficient hepatocytes

Sustained liver function and compensatory signaling in adult Mtu1LKO mice

Discussion

Materials and Methods

Animals

Primary hepatocyte culture

Gene expression analysis

Western blotting

Statistics

Supporting Information

S1 Fig. Morphological examination of liver-specific Mtu1 knockout mice.

S2 Fig. Relative amount of modifications at 34U.

S3 Fig. Sulfur-containing tRNA modifications in Mtu1LKO mice.

S4 Fig. Glutathione and glutathione disulfide levels in Mtu1LKO mice.

S5 Fig. Codon usage in mouse and human mitochondrial genes.

S1 Text. Supplemental Methods.

Acknowledgments

Author Contributions

References

Mtu1-mediated s² modification is essential for mitochondrial translation

Sustained liver function and compensatory signaling in adult Mtu1^LKO mice

S3 Fig. Sulfur-containing tRNA modifications in Mtu1^LKO mice.

S4 Fig. Glutathione and glutathione disulfide levels in Mtu1^LKO mice.