Toll like receptor 4 gene Asp299Gly polymorphism increases the risk of diabetic microvascular complications: a meta analysis

Diabetic microvascular complications (DMI) are the most common chronic complications of diabetes, which are the main causes of disability and death in diabetic patients [1], including diabetic retinopathy, diabetic nephropathy and diabetic neuropathy [2]. Many risk factors play an important role in the onset of DMI, such as course of diabetes, blood glucose control level, BMI and age [3, 4]. However, DMI are a complex metabolic disease composed of multiple factors including genetic and environmental factors, its specific pathogenesis is still unclear, causing difficult in diagnosis and treatment. Due to the high morbidity and mortality of DMI, early diagnosis and treatment are particularly important. Recent studies have shown that some macromolecules such as homocysteine (HCY), troponin T (TnT) and asymmetric dimethylarginine (ADMA) play an important part in the pathogenesis of diabetic vascular diseases, which have good clinical diagnostic value and can be considered as diagnostic markers for diabetic vascular complications [5‐7]. These macromolecules are more widely used in diagnosis of diabetic macrovascular complications, however, are less in DMI. Therefore, the discovery of biomarkers for the diagnosis of DMI requires further investigation. A cross-sectional retrospective study involving 90 patients showed that the expression of TLR4 in Diabetic polyneuropathy (DPN) patients was significantly higher than that in T2DM patients and healthy controls, and the up-regulation of TLR4 level would significantly increase the risk of DPN, which suggest that TLR4 may be a potential and sensitive diagnostic biomarker for diabetic neuropathy [8].

TLR4 gene, encodes TLR4 protein, located on chromosome 9Q32-33 and its variations can alter TLR4's recognition and interaction functions [9]. TLR4 is considered a key member of the TLRs families, as a highly conserved pattern recognition receptor, which can bind to specific ligands that induces activation of nuclear factor-κB, leading to an increase in downstream proinflammatory cytokines and adhesion molecules, involved in the occurrence of inflammatory responses by MyD88 dependent or non-dependent signaling pathways [10, 11]. The polymorphism of TLR4Asp299Gly gene may affect ligand binding, folding efficiency, cell surface expression and protein stability, while the polymorphism of Thr399Ile gene has little effect [12].

Recently, studies on the relationship between TLR4 gene polymorphism and type 2 diabetes mellitus (T2DM) and its complications have attracted extensive attention. Yin et al. indicated that TLR4 gene Asp299Gly and Thr399Ile polymorphisms are not associated with increased T2DM risk through a meta-analysis [13], whereas Chang et al. pointed out some problems that still exist or need to be improved in the meta-analysis of Yin et al. [14]. Several studies have shown that TLR4 gene polymorphism is associated with the occurrence of DMI, among which the research on TLR4Asp299Gly is the hotspot [15‐24]. Khaghanzadeh et al. [15] showed that c.1196C > T and 896A > G variants might increase the risk of DR by involving in the dysregulation of serum lipid levels and hyperglycemia. Buraczynska et al. [16] concluded that the G(rs4986790) polymorphism of TLR4Asp299Gly allele increased the risk of DR. That is to say, a significant increase of G allele frequency was observed in DR compared to those without it in T2DM (OR = 2.12, 95% CI (1.43–3.12), p = 0.0002). Yet Balistreri et al. [17] revealed that there was no correlation between rs4986790 gene polymorphism and the occurrence of DR and diabetic neuropathy. In view of the conclusions on the correlation between p.Asp299Gly and DMI are not consistent, so we performed this meta analysis to further study the relationship between them, to determine whether TLR4 gene polymorphism can be considered as a risk factor or diagnostic marker for DMI.

TLR4, as one of the key members of the earliest and most clearly studied Toll-like Receptors (TLRs) family, consists of extracellular domain, transmembrane domain and intracellular domain. The extracellular domain of 22 leucine-rich repeats mediates Lipopolysaccharide (LPS) recognition and receptor dimerization, while the intracellular domain is structurally similar to interleukin 1(TIR1) and plays an important role in downstream signal transduction [25]. TLR4 is mainly distributed on the surface of B lymphocytes, monocytes/macrophages, smooth muscle cells, dendritic cells and other cells [26]. As a highly conserved pattern recognition receptor, it can interact with endogenous ligands such as Heat shock protein(HSP), fibrinogen, High Mobility Group Box 1 protein(HMGB1), Oxidized low density lipoprotein(OX-LDL) and exogenous ligands such as LPS released by Gram-negative bacteria [27‐29]. The activation of Nuclear factor-kappa B(NF-κB) was induced by regulating the dependent or independent signaling pathways of Myeloid differentiation factor 88(MyD88) [30]. TLR4/MyD88/NF-κB signaling pathway leads to the increase of downstream pro-inflammatory cytokines and adhesion molecules, participate in the occurrence of inflammatory reactions [31], and cause the pathological changes such as vascular extravasation or increased vascular permeability, vascular obstruction, and degeneration and pathological changes of neovascularization, thus leading to the occurrence and development of DMI [32, 33]. Activation of the TLR4 signaling pathway mediates the inflammatory response, which is associated with TLR4 gene polymorphism [34]. Genetic variation of TLR4 can alter TLR4’s recognition and interaction functions, and then, change the immune response [9]. It has been reported that the replacement of the conserved Asp with Gly at position 299 theoretically cause disruption of the alpha helix protein structure, leading to extended beta strain, which is less functional [35]. As one of the most common variants of TLR4, Asp299Gly gene polymorphism is known to alter the extracellular domain of the receptor, resulting in hyporesponsiveness to LPS, attenuating the TLR4 signaling pathway and reducing the inflammatory response to Gram-negative pathogens [36, 37]. In addition, Zaharieva et al. also noted that it is mainly Asp299Gly rather than Thr399Ile polymorphism that leads to peptide structural modifications, changes in ligand-receptor interactions, post-receptor signal transduction, and further cytokine production [18].

Several studies have shown that TLR4 gene polymorphism is closely related to the occurrence and development of DMI [15‐24]. Multiple loci of the TLR4 gene polymorphisms such as rs4986791, rs1927911, rs1927914, rs10759931, are associated with DMI. What’s more, the relationship between TLR4Asp299Gly gene polymorphism and DMI is a hot topic [15‐21, 23]. The mutant of TLR4Asp299Gly/Thr399Ile will change the structure of TLR4 itself, leading to problems in ligand binding. This structural/functional irregularity seems ultimately to lead to a blunt immune response, such as the reduction of IgA production against microbial targets and the decrease of functional TLR4 levels [38]. The results of our meta analysis covering a total of 1834 cases and 4069 controls showed that TLR4Asp299Gly gene polymorphism increased the risk of DMI under dominant model and allele model (OR = 1.52, 95% CI (1.10–2.09), p = 0.01; OR = 1.42, 95% CI (1.02–1.96), p = 0.04 respectively). However, we found that there was no correlation between them under the recessive model and additive model (OR = 1.87, 95% CI (0.78–4.46), p = 0.16; OR = 1.94, 95% CI (0.81–4.61), p = 0.14 respectively). The conclusion of Carmela, CS Aioanei and Gottfried were contradictory to our results, which may be attributed to the ethnic difference of the included population and the difference of DMI types [17, 21, 23].

So it is necessary to perform subgroup analysis, we found that the significant association was observed in DR subgroup under dominant model and allele model (OR = 1.81, 95% CI (1.04–3.14), P = 0.03; OR = 1.77, 95% CI (1.05–2.98), P = 0.03 respectively) from subgroup analysis of the difference of DMI types. Nevertheless, no significant association was observed between TLR4Asp299Gly gene polymorphism and DN and diabetic neuropathy subgroup (p > 0.05). The studies of Buraczynska et al. [16], Buraczynska et al. [18], and Zaharieva [20] were consistent with our results, which further confirmed that TLR4Asp299Gly gene polymorphism was significantly associated with increased risk of DR. Therefore, we can infer that although DR, DN and diabetic neuropathy were included in microvascular complications, there still exists some differences in the pathogenesis.

To our knowledge, this is the first meta-analysis to investigate the relationship between TLR4Asp299Gly gene polymorphism and DMI. The results showed that TLR4Asp299Gly gene polymorphism increased the risk of retinopathy in patients with T2DM(dominant model OR = 1.81, 95% CI (1.04–3.14), P = 0.03; allelic model OR = 1.77, 95% CI (1.05–2.98), P = 0.03), but there was no correlation between this gene polymorphism and DN or diabetic neuropathy(DN: dominant model OR = 1.19, 95% CI (0.81–1.74), P = 0.38; allelic model OR = 0.91, 95% CI (0.50–1.64), P = 0.75; diabetic neuropathy: dominant model OR = 1.42, 95% CI (0.76–2.67), P = 0.27; allelic model OR = 1.40, 95% CI (0.80–2.44), P = 0.24). Hence, we speculated that the expression of TLR4 or its ligands in retinal vessels, glomerular microvessels and neural tissues may exist tissue specificity, and TLR4/MyD88/NF-κB inflammatory response regulated by signal channels may have the greatest effect on retinal vessels. From this we can put forward a hypothesis: TLR4Asp299Gly gene polymorphism may be a susceptibility indicator of DR and the detection of this susceptibility gene can be used as a clinical diagnostic index, which may be a new target for drug therapy of DR in the future.

A number of studies have found that distribution of TLR4Asp299Gly site is population specificity. African populations have the highest Asp299Gly mutation rates, and then Caucasians, and the probability of mutation in Asian population, especially in Chinese Han population, is very low [39‐41]. The study in Zhao et al. [42] found no genetic variation in Asp299Gly and Thr399Ile in Chinese Han populations, which is consistent with Huayin Cai’s findings [11]. Because TLR4Asp299Gly gene polymorphism varies widely among races, we performed a subgroup analysis of different ethnic groups in terms of Caucasian and Asian populations. The results showed that TLR4Asp299Gly gene polymorphism was associated with increased risk of DMI in Caucasian patients with T2DM under dominant model and allele model (dominant model OR = 1.69, 95% CI (1.22–2.35), P = 0.002; allelic model OR = 1.56, 95% CI (1.10–2.21), P = 0.01). This gene polymorphism may be a risk factor for DMI in the Caucasian population. Therefore, it may be used as a target for early prevention and treatment. But in the Asian population we found no correlation (dominant model OR = 0.85, 95% CI (0.52–1.39), P = 0.52; allelic model OR = 0.89, 95% CI (0.56–1.39), P = 0.60). This further confirmed that there are racial differences in TLR4Asp299Gly gene polymorphism. It's worth noting that the absence of GG genotype of TLR4Asp299Gly in some studies [15, 17, 20], So not all studies were included in recessive model and additive model analysis, which may have a certain impact on our final results.

Furthermore, we performed sensitivity analysis. The results showed that the corresponding OR value did not change significantly after the combination under the dominant model, which suggested that the overall results were statistically robust under this genetic model. However, the merge OR value and 95% CI (OR = 0.95, 95% CI (0.72–1.25), P = 0.70; heterogeneity: P = 0.81, I² = 0) were significantly altered under the allelic model and the heterogeneity disappeared, suggesting that the heterogeneity among the meta-included studies may be attributed to these studies which are excluded by us. At the same time, we can conclude that there was no correlation between TLR4Asp299Gly gene polymorphism and DMI in the allelic model after sensitivity analysis.

In order to explain the results obtained better, some limitations of this meta-analysis should not be ignored. Firstly, DMI are a complex metabolic disease with multiple genetic and environmental factors. This meta analysis does not take into account the effects of other loci of TLR4 gene or other susceptible genes polymorphisms and environmental factors. Secondly, some studies have shown that glycated albumin(GA) can be used as a predictor of diabetes, its microvascular complications and cardiovascular prognosis compared with fasting glucose(FPG) and glycated hemoglobin(HbA1c), and it would be more convincing if GA was detected in our meta-included studies[43, 44]. Thirdly, there was heterogeneity among the studies included in the dominant and allelic model analysis. The heterogeneity was not completely eliminated by subgroup analysis with different race and difference of DMI types and sensitivity analysis.

In conclusion, this meta analysis showed that TLR4Asp299Gly gene polymorphism was associated with increased risk of DMI under dominant model, while no significant correlation was observed under allelic model, recessive model and additive model. TLR4Asp299Gly gene polymorphism may be considered as one of the risk factors for DMI. More importantly, our study have shown that this gene polymorphism increased the risk of DR in patients with T2DM, but not DN or diabetic neuropathy. Therefore, the detection of TLR4Asp299Gly can be used as a clinical diagnostic index and may be a new target for drug therapy of DR in the future.