Basic Study Open Access
Copyright ©The Author(s) 2024. Published by Baishideng Publishing Group Inc. All rights reserved.
World J Diabetes. Aug 15, 2024; 15(8): 1753-1763
Published online Aug 15, 2024. doi: 10.4239/wjd.v15.i8.1753
Functional analysis of the novel mitochondrial tRNATrp and tRNASer(AGY) variants associated with type 2 diabetes mellitus
Yu Ding, Qin-Xian Guo, Jian-Hang Leng, Central Laboratory, Hangzhou First People’s Hospital, Hangzhou 310006, Zhejiang Province, China
Xue-Jiao Yu, Clinical Laboratory, Quzhou People’s Hospital, Quzhou 324000, Zhejiang Province, China
ORCID number: Yu Ding (0000-0003-1246-2563).
Co-first authors: Yu Ding and Xue-Jiao Yu.
Author contributions: Ding Y contributed to conceptualization; Ding Y and Yu XJ contributed to formal analysis; Ding Y, Guo QX, and Leng JH contributed to investigation; Ding Y and Yu XJ contributed to writing-original draft preparation; Ding Y contributed to writing-review and editing; and all authors have read and agreed to the published version of the manuscript.
Supported by the Hangzhou Joint Fund of the Zhejiang Provincial Natural Science Foundation of China, No. LHZY24H020002; Hangzhou Municipal Health Commission, No. ZD20220010; and Quzhou Bureau of Science and Technology, No. 2022K51.
Institutional review board statement: The study was reviewed and approved by the Ethics Committee of Hangzhou First People’s Hospital (Approval No. KY-20240327-0100-01).
Conflict-of-interest statement: The authors declare that they have no conflict of interest to disclose.
Data sharing statement: The datasets for this study will be available from the corresponding authors upon reasonable request.
Open-Access: This article is an open-access article that was selected by an in-house editor and fully peer-reviewed by external reviewers. It is distributed in accordance with the Creative Commons Attribution NonCommercial (CC BY-NC 4.0) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is non-commercial. See: https://creativecommons.org/Licenses/by-nc/4.0/
Corresponding author: Yu Ding, MD, Associate Professor, Central Laboratory, Hangzhou First People’s Hospital, No. 261 Huansha Road, Hangzhou 310006, Zhejiang Province, China. dingyu_zj@126.com
Received: February 15, 2024
Revised: May 9, 2024
Accepted: June 18, 2024
Published online: August 15, 2024
Processing time: 162 Days and 0 Hours

Abstract
BACKGROUND

Mutations in mitochondrial tRNA (mt-tRNA) genes that result in mitochondrial dysfunction play important roles in type 2 diabetes mellitus (T2DM). We pre-viously reported a large Chinese pedigree with maternally inherited T2DM that harbors novel mt-tRNATrpA5514G and tRNASer(AGY)C12237T variants, however, the effects of these mt-tRNA variants on T2DM progression are largely unknown.

AIM

To assess the potential pathogenicity of T2DM-associated m.A5514G and m.C12237T variants at genetic, molecular, and biochemical levels.

METHODS

Cytoplasmic hybrid (cybrid) cells carrying both m.A5514G and m.C12237T variants, and healthy control cells without these mitochondrial DNA (mtDNA) variants were generated using trans-mitochondrial technology. Mitochondrial features, including mt-tRNA steady-state level, levels of adenosine triphosphate (ATP), mitochondrial membrane potential (MMP), reactive oxygen species (ROS), mtDNA copy number, nicotinamide adenine dinucleotide (NAD+)/NADH ratio, enzymatic activities of respiratory chain complexes (RCCs), 8-hydroxy-deo-xyguanine (8-OhdG), malondialdehyde (MDA), and superoxide dismutase (SOD) were examined in cell lines with and without these mt-tRNA variants.

RESULTS

Compared with control cells, the m.A5514G variant caused an approximately 35% reduction in the steady-state level of mt-tRNATrp (P < 0.0001); however, the m.C12237T variant did not affect the mt-tRNASer(AGY) steady-state level (P = 0.5849). Biochemical analysis revealed that cells with both m.A5514G and m.C12237T variants exhibited more severe mitochondrial dysfunctions and elevated oxidative stress than control cells: ATP, MMP, NAD+/NADH ratio, enzyme activities of RCCs and SOD levels were markedly decreased in mutant cells (P < 0.05 for all measures). By contrast, the levels of ROS, 8-OhdG and MDA were significantly increased (P < 0.05 for all measures), but mtDNA copy number was not affected by m.A5514G and m.C12237T variants (P = 0.5942).

CONCLUSION

The m.A5514G variant impaired mt-tRNATrp metabolism, which subsequently caused mitochondrial dysfunction. The m.C12237T variant did not alter the steady-state level of mt-tRNASer(AGY), indicating that it may be a modifier of the m.A5514G variant. The m.A5514G variant may exacerbate the pathogenesis and progression of T2DM in this Chinese pedigree.

Key Words: Type 2 diabetes mellitus; Mitochondrial tRNA genes; Novel variants; Oxidative stress; Mitochondrial dysfunctions

Core Tip: We established cytoplasmic hybrid (cybrid) cells with m.A5514G and m.C12237T variants, and control cells without these variants. The m.A5514G variant decreased mt-tRNATrp stability, whereas the m.C12237T variant did not alter the stability of mt-tRNASer(AGY). More severe mitochondrial dysfunction was observed in mutant cybrids than in control cells, indicating that the m.A5514G variant impaired mt-tRNATrp metabolism and mitochondrial functions and increased cellular oxidative stress, which play central roles in type 2 diabetes mellitus (T2DM) progression. By contrast, the m.C12237T variant acted as a modifier of the m.A5514G variant. Our study provides novel insight into the pathophysiology of maternally transmitted T2DM caused by novel mt-tRNA variants.



INTRODUCTION

Diabetes is a common endocrine disease caused by the presence of chronic hyperglycemia. This complex disorder can be divided into type 1 and type 2. Type 2 diabetes mellitus (T2DM) is a major public health problem that affects approximately 10% of the Chinese adult population[1]. T2DM is characterized by high blood glucose in the context of insulin resistance (IR) and relative insulin deficiency. Furthermore, T2DM-associated complications, such as cardiovascular and peripheral vascular diseases, diabetic retinopathy, foot problems and nephropathy, remain very big challenge for clinicians[2]. Tremendous progression has been made in understanding the pathophysiology of T2DM over the past decades[3-5], with both genetic variations and environmental factors being involved in T2DM pathogenesis[6,7]. Nevertheless, the early prevention, diagnosis, and treatment of T2DM remain far from satisfactory.

Deregulation of mitochondrial oxidative phosphorylation (OXPHOS) is widely accepted as a major cause of T2DM and IR[8], diminished OXPHOS contributes to IR through elevated reactive oxygen species (ROS) production, and disrupted insulin receptor signaling[9]. Mitochondria are present in most eukaryotic cells and their primary role is to provide energy in the form of adenosine triphosphate (ATP) via OXPHOS[10]. They have their own DNA, mitochondrial DNA (mtDNA), which is 16569-bp in length and encodes 13 polypeptides, two rRNAs and 22 tRNAs[11]. Although mt-tRNA genes account for only approximately 10% mitochondrial genome, more than two third of mitochondrial disease-related variations are localized in this region[12]. An early landmark discovery in T2DM research was the identification of a 10.4-kb large deletion in mtDNA[13] and the m.A3243G mutation in mt-tRNALeu(UUR)[14]. A growing number of mtDNA variants has since been reported, for example, mt-tRNAGlu A14692G[15], mt-tRNAThr G15897A[16] and mt-tRNAGly T10003C[17] are potential pathogenic variants affecting T2DM predisposition. Exactly how these mt-tRNA variants contribute to disease onset, however, remains poorly understood, and, there is an urgent need for additional studies to determine how mitochondrial dysfunction mediates the onset or progression of T2DM.

To understand the molecular basis of mitochondrial diabetes and to provide valuable information for its diagnosis, prevention, and treatment, we previously performed a systematic and extended screen for mt-tRNA gene variants in a cohort of 370 Chinese patients with T2DM and 631 healthy controls who were recruited from Hangzhou First People’s Hospital and Quzhou People’s Hospital in Zhejiang Province of China. We showed that mt-tRNALeu(UUR) A3243G, ND6 T14502C[18], ND4 G11696A[19], ND5 T12338C and mt-tRNAAla T5587C variants[20] are involved in the pathogenesis of maternally inherited T2DM. More recently, we reported a large Chinese pedigree with maternally transmitted T2DM, intriguingly, among 18 matrilineal relatives of this pedigree, six individuals suffered from diabetes. The age at T2DM onset ranged from 40 to 70 years, with an average of 52 years. Mutational analysis of nuclear genes (GJB2, GJB3, GJB6, and TRMU) indicated no functional variants. Sequence analysis of entire mitochondrial genomes in matrilineal relatives revealed the presence of novel mt-tRNATrpA5514G and mt-tRNASer(AGY)C12237T variants[21]. The m.A5514G variant disrupted a highly conserved base-pairing (3A-70T) in the Acceptor arm of mt-tRNATrp, whereas the m.C12237T variant created a novel Watson-Crick base-pairing (11A-31T) in the Variable region of mt-tRNASer(AGY) (Figure 1). We therefore hypothesized that change in the mt-tRNATrp and mt-tRNASer(AGY) secondary structures caused by the m.A5514G and m.C12237T variants caused aberrant mt-tRNA metabolism which led to mitochondrial dysfunction and T2DM progression[22]. However, the pathophysiology of T2DM-related m.A5514G and m.C12237T variants remains largely undetermined.

Figure 1
Figure 1 The secondary structures of mitochondrial tRNATrp and mitochondrial tRNASer(AGY), arrows indicated the positions of the m.A5514G and m.C12237T variants. mt-tRNA: Mitochondrial tRNA.

To elucidate the pathogenic mechanism of the novel mt-tRNATrp and mt-tRNASer(AGY) variants, we generated cybrid cell lines derived from four T2DM patients carrying both m.A5514G and m.C12237T variants, together with four cybrids derived from control subjects without these mtDNA variants but belonging to the same mtDNA haplogroup. We examined whether the m.A5514G and m.C12237T variants affected mt-tRNA steady-state levels by northern blotting, and evaluated mitochondrial characteristics including levels of mtDNA copy number, malondialdehyde (MDA), superoxide dismutase (SOD), 8-hydroxy-deoxyguanine (8-OhdG), ATP, mitochondrial membrane potential (MMP), ROS, nicotinamide adenine dinucleotide (NAD+)/NADH ratio and respiratory chain complexes (RCCs) activities in the mutant and control cybrids.

MATERIALS AND METHODS
Subjects

Members of a Han Chinese family with T2DM were enrolled via Hangzhou First People’s Hospital as a part of genetic screening program for T2DM-associated mtDNA novel variants, as described previously[21]. The protocol used in this investigation was in accordance with the principles expressed in the 1975 Declaration of Helsinki, revised in 2008. The Ethics Committee of Hangzhou First People’s Hospital approved this study (No. KY-20240327-0100-01). All participants, including four affected matrilineal relatives with T2DM (III-5, III-10, III-18, and III-22) bearing the m.A5514G and m.C12237T variants, belonged to mtDNA haplogroup G2a according to East Asian phylogeny[23]. Four genetically unrelated healthy subjects (C1, C2, C3, and C4) lacking these mt-tRNA variants and also belonging to human mtDNA haplogroup G2a were selected as controls. Written informed consent for participating in this study and for publication of case details was obtained from all subjects enrolled in the study.

Generation of cybrid cell lines

Cybrid cells can incorporate human mitochondria and perpetuate the mtDNA-encoded components of the incorporated mitochondria, which keeping the nuclear background constant[24]. To generate cybrids, the platelets of four patients with both m.A5514G and m.C12237T variants (III-5, III-10, III-18, and III-22), together with four controls (C1, C2, C3, and C4) were fused with 143B-ρ0 206 cells, as described previously[25]. The 143B-ρ0 206 cells were grown in DMEM (Thermo Fisher Scientific, Waltham, MA, United States) supplemented with 10% FBS (Sigma, Aldrich, St. Louis, MO, United States) and 50 µg/mL uridine. The cybrid transformants were cultured in high-glucose DMEM containing 10% FBS at 37 °C in a humidified CO2 incubator.

To determine successful construction of cybrids, PCR-Sanger sequencing was performed to examine the presence of the m.A5514G and m.C12237T variants. The primer for amplification of the mt-tRNATrp gene were: Forward, 5’-CTA ACC GGC TTT TTG CCC-3’; reverse: 5’-ACC TAG AAG GTT GCC TGG CT-3’. The primers for amplification of the mt-tRNASer(AGY) gene were: forward, 5’-TAT CAC TCT CCT ACT TAC AG-3’; reverse: 5’-AGA AGG TTA TAA TTC CTA CG-3’. The PCR products were purified, sequenced and compared with an updated version of the human mitochondrial genome sequence to detect the variants (GenBank Accessible No: NC_012920.1)[26].

Northern blot analysis

Total mitochondrial RNA was obtained from mitochondria isolated from mutant and control cybrid cell lines (approximately 2 × 108 cells) using the TOTALLY RNATM kit (Ambion, Thermo Fisher Scientific), as described previously[27]. For northern blotting analysis of mt-tRNA, 2 µg of total mitochondrial RNA was electrophoresed through a 10% polyacrylamide/8M urea gel in Tris borate-EDTA buffer. The sequences for digoxigenin (DIG)-labeled probes specific to mt-tRNATrp; mt-tRNASer(AGY) and 5S rRNA were: 5’-AGA AAT TAA GTA TTG CAA CTT ACT GAG GGC-3’; 5’-GAG AAA GCC ATG TTG TTA GAC ATG GGG GCA-3’ and 5’-GGG TGG TAT GGC GGT AGA C-3’, respectively. Hybridization and quantification of band density were performed as previously described[28].

Analysis of ATP levels

The CellTiter-Glo® luminescent cell viability assay (Promega, Madison, WI, United States) was used to measure ATP levels in mutant and control cybrids according to the manufacturer’s instructions[29]. Cells were seeded into white 96-well plates at 1 × 105 cells per well and cultured for 20 hours to reach approximately 70% confluence. Cells were then lysed by the addition of 100 μL CellTiter-Glo® working solution to each well and incubation for 2 minutes in the dark. Cell lysate solution (200 μL) was then transferred to an opaque 96-well plate. A 200 μL solution of culture medium and working solution at a ratio of 1:1 was used as a control. ATP concentration was determined using a 96-well fluorescence detector.

MMP analysis

The JC-1 MMP Assay Kit (Abcam, United States) was used to detect MMP in mutant and wild type cell lines. The JC-1 dye fluoresces in healthy cells with high levels of MMP, and green in cells with low levels of MMP[30]. JC-1 probe (1 µg/mL) was added to approximately 1 × 105 cells and incubated for 30 minutes in the dark. Cells were then washed twice with PBS and immediately analyzed by FACSCanto II flow cytometry (BD Biosciences, United States).

Analysis of mitochondrial ROS production

Mutant and control cybrid cells were seeded in 6-well plates (1 × 105 cells/well) and loaded with 10 µmol/L 2’,7’-dichlorofluorescein diacetate (DCFH-DA, Beyotime, China) at 37 °C for 20 minutes. Cells were then washed with PBS three times and subsequently evaluated by FACSCanto II flow cytometry (BD Biosciences, United States).

Determination of NAD+/NADH ratio

The NAD+/NADH ratio is a measure of global energy capacity because the activities of rate-limiting enzymes involved in the tricarboxylic acid cycle (TCA), ketone production and glycolysis are regulated by this ratio[31,32]. The NAD+/NADH ratio was determined for 1 × 105 cells using the NAD+/NADH Assay Kit (Abcam, Cambridge, United Kingdom) ac-cording to the manufacturer’s instructions. Standard curves were generated for quantification.

Determination of mtDNA copy number

mtDNA copy number was determined using a quantitative real-time PCR (qRT-PCR) method, as described elsewhere[33]. Genomic DNA was extracted from 3 mL of blood from each participant using a QIAamp DNA Blood Mini Kit (Qiagen, Hilden, Germany) according to the manufacturer’s protocol. For qRT-PCR analysis, 100 ng genomic DNA was used as template. The primers specific for the mtDNA-ND1 gene were: Forward, 5’-CCTAGC CGT TTA CTC AAT CCT-3’; reverse: 5’-TGA TGG CTA GGG TGA CTTCAT-3’; the primer sequences for nuclear (hemoglobin) gene were: forward, 5’-GCT TCT GAC ACA ACT GTG TTC ACT AGC-3’; reverse: 5’-CAC CAA CTT CAT CCA CGT TCA CC-3’. The qRT-PCR reaction was performed on an ABI 7900 instrument (Thermo Fisher Scientific) using SYBR Green Realtime PCR Master Mix (Bioteke, China). Relative expression levels were normalized by the 2-ΔΔCT method[34]. Samples were assayed in triplicate.

Analysis of oxidative stress-related biomarkers

To determine the effects of the m.A5514G and m.C12237T variants on oxidative stress[35], the concentrations of MDA and SOD in four cybrids with the m.A5514G and m.C12237T variants (III-5, III-10, III-18, and III-22), and in four control cell lines (C1, C2, C3, and C4) were analyzed using colorimetric assay kits (Nanjing Jiancheng Bioengineering Institute, Nanjing, China). The serum levels of 8-OhdG were quantified by a competitive enzyme linked immunosorbent assay (ELISA) according to the manufacturer’s protocol (Nikken Foods, St. Louis, MO, United States). Samples were assayed in triplicate.

Analysis of enzymatic activities of mitochondrial RCCs

RCCs comprise four enzyme complexes (I-IV), which are embedded in the inner mitochondrial membrane and catalyze the transfer of reducing equivalents from high energy compounds. To analysis the activities of respiratory chain enzymes, an enriched mitochondrial fraction was isolated from mutant and control cybrid cells by centrifugation, as described previously[36]. The protein concentration was determined using a BCA protein assay kit (Thermo Fisher Scientific, Waltham, MA, United States). The enzymatic activities of RCCs were assayed spectrophotometrically, and the results were normalized to the activity of citrate synthase, a mitochondrial matrix enzyme[37].

Redefining the pathogenic roles of the m.A5514G and m.C12237T variants

We used the revised pathogenicity scoring system for mt-tRNA variants proposed by Yarham et al[38]. This scoring system gives special weight to functional data, which are considered the gold standard methods for assigning pathogenicity. The scoring system was as follows: ≤ 6 points, neutral polymorphism; 7-10 points, possibly pathogenic; 11-13 points (not including evidence from single-fiber, steady-state level, or trans-mitochondrial cybrid studies), probably pathogenic; ≥ 11 points (including evidence from single fiber, steady-state level or trans-mitochondrial cybrid studies), definitely pathogenic.

Statistical analysis

Data are presented as the mean ± SD. Statistical analysis of results was performed using GraphPad Prism 9.0 software (GraphPad. Software Inc., La Jolla, CA, United States). Student’s t-test or the Mann-Whitney test were used to assess the difference between two groups. A P value less than 0.05 was considered statistically significant.

RESULTS
Pedigree information and establishment of cybrid cell lines

We previously described a large Han Chinese pedigree with maternally transmitted T2DM that harbors the mt-tRNATrp A5514G and mt-tRNASer(AGY) C12237T variants[21]. Six individuals (one man and five women) of 18 matrilineal relatives suffered from T2DM. The age at onset varied among these six individuals from 40 to 70 years, with an average of 52 years.

To analyze mitochondrial functions, cybrid cell lines were derived from four subjects (III-5, III-10, III-18, and III-22) aged < 50 and from four genetically unrelated healthy subjects (C1, C2, C3, and C4) belonging to the same mtDNA haplogroup for use as controls. The platelets of these subjects were fused with the mtDNA-less human ρo206 cell line and cybrid clones were isolated by growing in selective DMEM, according to a previously described protocol[25]. The cybrid cell lines were analyzed by direct sequencing for the presence of the m.A5514G and m.C12237T variants and for homo-plasmy.

mt-tRNA analysis

To investigate whether the m.A5514G and m.C12237T variants perturbed mt-tRNA metabolism, we subjected mt-RNAs from mutant and control cell lines to northern blotting and hybridized them with DIG-labeled oligodeoxynucleotide probes for mt-tRNATrp and mt-tRNASer(AGY). As shown in Figure 2A, the steady-state level of mt-tRNATrp in mutant cell lines was significantly decreased, whereas the steady-state level of mt-tRNASer(AGY) was not affected in either mutant or wild type cells. For comparison, the m.A5514G variant caused approximately 35% reduction in the level of mt-tRNATrp (P < 0.0001) after normalization of 5S rRNA, however, the m.C12237T variant had little impact on the mt-tRNASer(AGY) steady-state level (P = 0.5849) (Figure 2B).

Figure 2
Figure 2 Analysis of steady-state levels of mitochondrial tRNATrp and mitochondrial tRNASer(AGY) by Northern blotting. A: 2 µg mitochondrial tRNA (mt-RNA) were electrophoresed through a denaturing polyacrylamide gel and hybridized with DIG-labeled oligonucleotide probes for mt-tRNATrp, mt-tRNASer(AGY), and 5S rRNA; B: Qualification of mt-tRNA levels.
ATP levels are decreased in m.A5514G and m.C12237T cybrid cells

We next assessed whether the variants influenced ATP generation by using a luciferin/Luciferase assay. As shown in Figure 3A, the average levels of ATP production in mutant cells decreased approximately 22.1% compared with control cells (P = 0.0016).

Figure 3
Figure 3 Analysis of mitochondrial functions in mutant and control cybrids. A: Adenosine triphosphate analysis; B: Mitochondrial membrane potential levels; C: Reactive oxygen species analysis; D: Nicotinamide adenine dinucleotide/NADH ratio; E: Mitochondrial DNA copy number; F: 8-hydroxy-deoxyguanine levels; G: Malondialdehyde levels; H: Superoxide dismutase levels. ATP: Adenosine triphosphate; MMP: Mitochondrial membrane potential; ROS: Reactive oxygen species; NAD: Nicotinamide adenine dinucleotide; mtDNA: Mitochondrial DNA; 8-OhdG: 8-hydroxy-deoxyguanine; MDA: Malondialdehyde; SOD: Superoxide dismutase.
The m.A5514G and m.C12237T variants reduce the levels of MMP

The effects of m.A5514G and m.C12237T variants on MMP was measured using the fluorescence probe, JC-1, in control and mutant cells. The relative ratios of the FL590/FL529 geometric means between control and mutant cells were assessed to depict the MMP level. As shown in Figure 3B, cells carrying mt-tRNA variants had 25.6% less MMP compared with control cells (P < 0.0001).

ROS production is enhanced in m.A5514G and m.C12237T cybrid cells

We used flow cytometry and DCFH-DA probe loading to assess ROS production in mutant and control cell lines. As shown in Figure 3C, mutant cells bearing the m.A5514G and m.C12237T variants exhibited increased ROS production, with an average increase of 127.5% relative to control cells (P < 0.0001).

The NAD+/NADH ratio is decreased in m.A5514G and m.C12237T cybrid cells

The NAD+/NADH ratio is involved in central carbon metabolism, nucleotide synthesis and lipid metabolism[39]. We measured the NAD+/NADH ratio in mutant and control cell lines and demonstrated that the mt-tRNA variants significantly reduced the NAD+/NADH ratio (Figure 3D).

mtDNA copy number is not affected by m.A5514G and m.C12237T variants

mtDNA copy number is a biomarker for both mitochondrial quality and function[40]. We therefore analyzed the mtDNA content in peripheral blood. As shown in Figure 3E, there were no differences in mtDNA copy number among patients with the m.A5514G and m.C12237T variants and controls (P = 0.5942).

Serum 8-OhdG levels are increased in T2DM individuals

8-OhdG, a critical biomarker of DNA damage, plays an important role in T2DM progression[41]. The concentrations of serum 8-OhdG in T2DM and control subjects were measured by ELISA. As shown in Figure 3F, patients with mt-tRNA variants had much higher concentrations of 8-OhdG compared with controls (P < 0.0001).

The m.A5514G and m.C12237T variants increase cellular oxidative stress

We next explored whether the mt-tRNA variants affected cellular oxidative stress. Individuals carrying the mt-tRNA variants showed much higher levels of MDA (P < 0.0001; Figure 3G) but significantly decreased levels of SOD (P = 0.0032) (Figure 3H) compared with controls.

The m.A5514G and m.C12237T variants inhibit the activities of Complex I and IV in cybrids

Mitochondrial Complex I is the major site for catalyzing oxidation of NADH. We therefore analyzed the enzyme activities of Complex I-IV in cybrids. As shown in Figure 4, the activities of Complex I and IV were dramatically inhibited (P < 0.0001, both), while Complex II and III enzyme activities remained unaffected (P = 0.5019 and 0.5523, respectively) in the m.A5514G and m.C12237T variants cybrids.

Figure 4
Figure 4 Analysis of enzymatic activities of mitochondrial respiratory chain complexes in four cybrids with mitochondrial tRNA variants and four control cell lines without these variants. C: Control group; M: Mutant group.
Pathogenicity of the m.A5514G and m.C12237T variants

Total scores of the m.A5514G and m.C12237T variants were 13 and 6 points, respectively, (Table 1), indicating that they were “definitely pathogenic” and “neutral polymorphism”, respectively.

Table 1 Redefining the pathogenic roles of the m.A5514G and m.C12237T variants.
Scoring criteria
m.A5514G variant
Score/20
m.C12237T variant
Score/20
Classification
More than one independent reportYes2Yes2≤ 6 points: Neutral polymorphisms; 7-10 points: Possibly pathogenic; 11-13 points (not including evidence from single fiber, steady-state level, or trans-mitochondrial cybrid studies): Probably pathogenic; ≥ 11 points (including evidence from single fiber, steady-state level or trans-mitochondrial cybrid studies): Definitely pathogenic
Evolutionary conservation of the base pairNo changes2No changes2
Variant heteroplasmyNo0No0
Segregation of the mutation with diseaseYes2Yes2
Biochemical defect in complex I, III, or IVYes2No0
Evidence of mutation segregation with biochemical defect from single fiber studiesNo evidence0No evidence0
Mutant mt-tRNA steady-state level or evidence of pathogenicity in trans-mitochondrial cybrid studiesStrong evidence5No evidence0
Maximum scoreDefinitely pathogenic13Neutral polymorphism6
DISCUSSION

In the present study, we investigated the causal roles of T2DM-related m.A5514G and m.C12237T variants at genetic, molecular, and biochemical levels. The m.A5514G variant was initially described in a neonatal patient with multiple RCC defects[42], and the m.C12237T variant was first reported in patients with Leber’s Hereditary Optic Neuropathy (LHON)[43]. Subsequently, we showed these variants to be associated with T2DM[21]. At the molecular level, the m.A5514G variant occurs at conventional position 3 in the Acceptor arm of mt-tRNATrp, which is highly conserved among species. Importantly, the m.A5514G variant abolishes the 3A-70T Watson-Crick base-pairing, which is important in recognizing its cognate tryptophanyl-tRNA synthetase during translation[44]. This causes misreading or misrecognition by RNase P[45]. Interestingly, the m.T7512C variant, which occurs at the same position as mt-tRNASer(UCN), was suggested to be associated with mitochondrial encephalomyopathy with lactic acidosis and stroke-like episodes (MELAS) and with myoclonic epilepsy with ragged red fibers (MERRF) overlap syndrome[46]. We therefore speculate that the m.A5514G variant, which is similar to the m.T7512C variant, may alter the stability of mutant mt-tRNATrp, as indicated by our northern blotting results. Indeed, the average steady-state level of mt-tRNATrp was significantly reduced to 35% of control levels, which is below the proposed threshold to produce a clinical phenotype associated with an mt-tRNA mutation[47]. These data lead us to believe that the m.A5514G variant impairs mt-tRNATrp metabolism.

Genetically, unlike other canonical mt-tRNAs, mt-tRNASer(AGY) is a highly unique tRNA in humans, lacking the entire D-loop structure[22]. In fact, the homoplasmic m.C12237T variant is located at position 31 in the Variable region of mt-tRNASer(AGY), which creates a new 11A-31T Watson-Crick base-pairing. Although RNA Fold (http://rna.tbi.univie.ac.at/cgi-bin/RNAWebSuite/RNAfold.cgi) predicted this variant to alter the secondary structure of mt-tRNASer(AGY)[21], functional data indicated no obvious difference in mt-tRNASer(AGY) steady-state levels between mutant and control cell lines, strongly indicating that the m.C12237T variant did not affect mt-tRNASer(AGY) metabolism. Therefore, the m.C12237T variant most probably acts as a modifier of the m.A5514G variant in T2DM.

The perturbed tertiary structure caused by the m.A5514G variant made the mutant mt-tRNATrp more unstable and led to aberrant mt-tRNA metabolism, significantly reducing the activities of Complex I and IV in mutant cells, which was consistent with the clinical phenotypes of the affected patients. As a result, the RCC deficiency caused by the m.A5514G and m.C12237T variants may result in down-regulated mitochondrial biogenesis and uncoupling of the oxidative pathway for ATP synthesis. Pancreatic beta cells have a high OXPHOS demand and would, therefore, be primarily affected[48]. In the current study, ATP production was reduced by 22.1% in mutant cells as compared with control cells. In addition, defectives OXPHOS complexes can result in impaired MMP production. Importantly, MMP is generated by proton pumps (Complex I, III, and IV), and is an essential in energy storage during OXPHOS[49]. The average MMP level in patients’ cells was only 74.4% of that in control cells. As a result, the defective OXPHOS in cells with mt-tRNA variants increased the production of ROS, 8-OhdG and MDA. Indeed, MDA is generated in the oxidative degradation of polyunsaturated lipids[50], whereas SOD is an antioxidant enzyme able to break down harmful oxygen molecules within cells and convert them into less toxic products[51]. Therefore, the increased oxidative damage and decreased antioxidant activity may be involved in the occurrence of oxidative stress. This would damage mitochondrial and cellular proteins, lipids, and nucleic acids via chemical modifications, including nitrosylation, peroxidation and carbonylation, and, in turn, promote pancreatic beta cell dysfunction and IR[52,53].

Reduced mtDNA copy number has been theoretically linked to increased oxidative stress via increased production of ROS[54]. Our data show no changes in mtDNA content in mutant and control groups. However, the precise mechanisms that led to variation in mtDNA copy number are uncertain and genetic and environmental factors have been hypothesized to interact to determine the number of mitochondria in a cell[55]. Therefore, although the m.A5514G and m.C12237T variants lead to mitochondrial dysfunctions, other factors such as nuclear background, restored the mtDNA content in the mutant cell lines.

Cellular NAD exists in two forms, oxidized (NAD+) and reduced (NADH). It plays essential roles in cellular redox reactions and is responsible for accepting high energy electrons and carrying them to the electron transport chain for the synthesis of ATP[56]. In diabetic patients, increased NADH levels cause reductive stress, which elevates ROS production and leads to IR and cell death[57]. In our study, mutant cell lines showed a marked decrease in the NAD+/NADH ratio indicating that the m.A5514G and m.C12237T variants increases oxidative stress and mitochondrial dysfunction.

CONCLUSION

Our findings indicate that the m.A5514G variant reduced the steady-state level of mt-tRNATrp, which affected tRNA metabolism and led to mitochondrial dysfunctions involved in T2DM pathogenesis, whereas the m.C12237T variant had little impact on mt-tRNASer(AGY) stability and was probably a polymorphism with neutral effect on the for expressivity of the m.A5514G variant-induced T2DM phenotype. Furthermore, the incomplete penetrance of T2DM and variable clinical phenotypes indicate that mt-tRNA variants are not sufficient to produce clinical phenotypes. Therefore, other factors, such as environmental factors, nuclear genes or epigenetic modification, may contribute to T2DM progression. The main limitation of this study was the relatively small sample size, and further studies including more T2DM patients are needed to verify our conclusions.

ACKNOWLEDGEMENTS

We thank Jeremy Allen (PhD) for editing a draft of this manuscript.

Footnotes

Provenance and peer review: Unsolicited article; Externally peer reviewed.

Peer-review model: Single blind

Specialty type: Genetics and heredity

Country of origin: China

Peer-review report’s classification

Scientific Quality: Grade B, Grade B

Novelty: Grade B, Grade B

Creativity or Innovation: Grade B, Grade B

Scientific Significance: Grade B, Grade B

P-Reviewer: Roomi AB; Yoshinaga K S-Editor: Chen YL L-Editor: A P-Editor: Chen YX

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