Forty individuals comprising 22 subjects suffering from PU and 18 healthy controls, were recruited for this study. Additionally, the 22 subjects with PU were diagnosed just after having hip fracture in our hospital. Tissue samples were collected from all subjects, and stored in −80°C for further analysis. Participants aged >90 years, malignant origin, psychiatric and obstetric patients, allergy to wound products were excluded from our study. All procedures and use of tissue samples were approved by the Ethics Committee of our institute, and participants or their first-degree relatives had already signed the informed consents before start of the experiment after all potential risk factors were carefully explained. The study was conducted according to the Declaration of Helsinki.

DNA extraction kit (Qiagen, Dusseldorf, Germary) was used to extract the DNA from peripheral blood samples in accordance with the manufacturer's protocol. PCR was used to amplify the DNA fragments including rs1056629. The PCR products were sequenced in forward direction, and TaqMan genotyping kit (Qiagen) and BLAST were used to determine the SNP genotypes. Each experiment was performed three times.

We search public online tool (http://www.bioguo.org) to find gene polymorphism in MMP9 3′UTR that might break the interaction between MMP9 and miRNA.

TRIzol reagent (Invitrogen, Carlsbad, CA, USA) was utilized to extract total RNA from BJ fibroblast cells and tissue samples according to the manufacturer's instructions. M-MLV (Invitrogen) was utilized to synthesize the first stranded cDNA from 2 µg total RNA in a 25 µl mixture following guideline suggested by vendor. Agarose gels (2%) with 5 mg/ml nucleic acid dye was utilized to electrophorese the PCR product, and AlphaEaseFC software (Genetic Technologies, Miami, FL, USA) was utilized to conduct expression analysis of MMP9. An iCycler iQ real-time PCR system (Bio-Rad Laboratories, Inc., Hercules, CA, USA) with SYBR Green Master Mix (QPK-201; Toyobo, Co., Ltd., Osaka, Japan) was utilized to perform real-time PCR, and the reaction was carried out at 95°C for 5 min, 45 cycles of (25 sec at 95°C; 20 sec at 60°C; 30 sec at 72°C). U6 RNA and GAPDH served as internal controls. 2^−ΔΔCt method was utilized to analyze the relative expression of miR-194-3p, miR-491, miR-1915-3p, miR-941 and MMP9 mRNA. Three independent experiments were repeated.

BJ fibroblast cells were obtained from Lonza (Basel, Switzerland), and RPMI-1640 medium (Gibco) containing 10% FBS (fetal bovine serum) (Sijiqing, Hangzhou, China) and 1% penicillin-streptomycin was utilized to culture these cells under a humid atmosphere with 5% CO₂/95% air at 37°C. Prior to transfection, cell were seeded into 96-well plates at a final density of 1×10⁵ per well, when the cells grewn to 80% confluence, they were co-transfected with miR-194-3p mimics/inhibitors, miR-491 mimics/inhibitors, miR-1915-3p mimics/inhibitors, miR-941 mimics/inhibitors using Lipofectamine 2000 (Invitrogen) according to the manufacturer's instructions. Three independent experiments were repeated.

PCR was performed to amplify fragment of MMP9 cDNA, and then PCR products were inserted into pGL3 vector (Promega Corp., Madison, WI, USA), then direct sequencing was adopted to confirm the accuracy. The QuikChange^® Lightning Site-Directed Mutagenesis kit (Agilent Technologies) was used to perform the single-base mutation in gene polymorphism located in binding site of miR-194-3p (A allele to C allele), miR-491 (A allele to C allele), miR-1915-3p (G allele to A allele) or miR-941 (G allele to A allele) in MMP9 3′UTR according to the manufacturer's instructions, and meanwhile QuikChange^® Lightning Site-Directed Mutagenesis kit (Agilent Technologies) with carefully designed primers was used to perform the miR-194-3p, miR-491, miR-1915-3p or miR-941 seed sequence mutation in MMP9 3′UTR. The above eight mutagenesis were performed for the same site and introduced to the pGL3 vector (Promega Corp.) at the same time, direct sequencing was adopted to confirm the mutation site accuracy. Three independent experiments were performed.

Full length of MMP9 3′UTR containing predicted binding site of miR-194-3p, miR-491, miR-1915-3p or miR-941 was amplified using PCR, then the above PCR products were inserted into pGL3-control vector (Promega Corp.), and located downstream of the luciferase gene, and obtained pGL3-MMP9-3′UTR construct. Then the ‘seed sequence’ in MMP9 3′UTR was mutated, and PCR was also performed to obtain point mutations, and cloned into pGL3-control vector (Promega Corp.) to generate pGL3-MMP9 3′UTR Mut construct. 1×10⁵ BJ fibroblast cells were seeded into 96-well plates for 24 h. Lipofectamine 3000 (Invitrogen) was utilized to transfect miR-194-3p, miR-491, miR-1915-3p or miR-941 mimic or NC (negative control) RNA oligonucleotide and 0.4 mg of pGL3 constructs along with 0.07 mg of pRL-CMV plasmid-expressing renilla luciferase into BJ fibroblast cells. Dual Luciferase Reporter assay system (Promega Corp.) was utilized to detect luciferase activity 48 h post-transfection, and luciferase activity of firefly was normalized to that of renilla luciferase. Three independent tests were repeated.

The total protein was extracted from BJ fibroblast cells and tissue samples using lysis buffer (Beyotime, Haimen, China), and Enhanced BCA Protein assay kit (Byotime) was utilized to measure protein concentration according to the manufacturer's instructions. Polyacrylamide gel (10%) (w/v) with SDS-PAGE was utilized to separate protein extracts, and then electro-transferred onto PVDF (polyvinylidene difluoride) (PerkinElmer, Waltham, MA, USA) membrane for 90 min. Non-fat milk (5%) was utilized to block the membrane. Then monoclonal antibodies against anti-human MMP9 (1:5,000; Abcam, Cambridge, MA, USA) at 1:12,000 dilution β-actin (Santa Cruz Biotechnology, Inc., Santa Cruz, CA, USA) were utilized to incubate the membranes for 12 h at 4°C, next, HRP (horse raddish peroxidase)-linked mouse anti-goat secondary antibody at 1:15,000 dilution (1:3,000, Santa Cruz Biotechnology, Inc.) was utilized to treat the membranes for another 1 h. The Fusion FX7 system (VilberLourmat, Marne-la-Vallée, France) with SuperSignal™ West Pico Chemiluminescent Substrate (Thermo Fisher Scientific, Inc., Waltham, MA, USA) was utilized to visualize the bands, and ImageJ Analyst software [National Institutes of Health (NIH), Bethesda, MD, USA) was utilized to quantify the level of MMP9. Three independent experiments were carried out.

Anti-MMP9 antibody (1:500; Abcam) was utilized to carry out immunohistochemistry for MMP9 on a 4-µm tissue sample. Xylene was utilized to bake and deparaffinize the slides, and graded alcohol was utilized to pass through the above slides, next 1 mM EDTA (Invitrogen) was utilized to retrieve antigen in a steam pressure cooker (Decloaking Chamber; BioCare Medical, Walnut Creek, CA, USA) for 30 sec at 125°C. The following experimentations were performed in a hydrated chamber at room temperature. Peroxidase Block (Dako, Carpentaria, CA, USA) was utilized to pretreat the slides for 5 min to quench the activity of endogenous peroxidase, and 50 mM Tris-Cl, pH 7.4 to wash the slides. 5 ml 50 mM Tris-Cl containing 250 µl normal goat serum (Dako) was utilized to block the slides, anti-MMP9 antibody (1:500; Abcam) to incubate the slides for 60 min. Tris-Cl (50 mM), pH 7.4 was utilized to wash the slides, rabbit HRP conjugated Signal stain boost IHC detection reagent (Cell Signaling Technology, Inc., Danvers, MA, USA) was utilized to treat the slides for 30 min, and Tris-Cl (50 mM), pH 7.4 to wash the slides, DAB (3,3′diaminobenzidine) chromogen (Dako) was utilized to develop immunoperoxidase staining for 5 min, followed by counterstaining with hematoxylin. Following staining, two experienced pathologists scored immunostaining independently, two pathologists were blinded to the clinical outcomes and clinicopathological parameters of the subjects. The scores of the two pathologists with any discrepancy were re-examining by both pathologists to obtain a consensus score.

The data are presented as means ± SD (standard deviation). GraphPad Prism 5.0 (GraphPad Software Inc. La Jolla, CA, USA) was utilized to perform the statistical analyses. Unpaired t-test was utilized for comparison of the result of real-time PCR. Chi-square test was employed to analyze qualitative data, and Pearson correlation analysis to determine the correlation. P<0.05 was considered to indicate a statistically significant difference.

We searched online miRNA database (http://www.bioguo.org) to identify the gene polymorphisms in MMP9 3′UTR that might potentially interfere with the interaction between MMP9 and miRNA, and found that gene polymorphism MMP9 3′UTR might compromise the interaction between MMP9 with miR-194-3p, miR-491, miR-1915-3p or miR-941, and QuikChange^® Lightning Site-Directed Mutagenesis kit (Agilent Technologies, CA, USA) was used to introduce the mutations (either the minor allele of the target polymorphism or the complementary sequence of the seed sequence) located in binding site of miR-194-3p (mutant-1 and mutant-2) (Fig. 1A), miR-491 (mutant-3 and mutant-4) (Fig. 1B), miR-1915-3p (mutant-5 and mutant-6) (Fig. 1C) and miR-941 (mutant-7 and mutant-8) (Fig. 1D) in MMP9 3′UTR according to the manufacturer's instructions.

Luciferase assay was performed to test whether miR-194-3p, miR-491, miR-1915-3p or miR-941 directly regulated MMP9 expression or the effect of the candidate polymorphism on the interaction between the miRNAs and MMP9. The cells were co-transfected with constructs containing wild-type MMP9 3′UTR and mutant-1–9 MMP9 3′UTR and miR-194-3p, miR-491, miR-1915-3p or miR-941 mimic. As shown in Fig. 2, only transfection with miR-491 (Fig. 2B) significantly reduced luciferase activity of wild-type MMP9 3′UTR, whereas luciferase activity of mutant-3 and mutant-4 MMP9 3′UTR showed no obvious difference in comparison with scramble control. By contrast, luciferase activity of co-transfected constructs containing wild-type MMP9 3′UTR and mutant-1/2/5/6/7/8 MMP9 3′UTR and miR-194-3p, miR-1915-3p or miR-941 mimic was comparable with scramble control, respectively. The results indicated that miR-491 directly targeted MMP9, and rs1056629 disrupted the interaction between MMP9 and miR-491.

Forty individuals comprising with (N=22) or without (N=18) PU were recruited for this study, and all those subjects were rs1056629 genotype. Real-time PCR was performed to detect expressions of miR-194-3p, miR-491, miR-1915-3p or miR-941 and MMP9 in these subjects. As shown in Fig. 3, miR-194-3p (Fig. 3A), miR-491 (Fig. 3C), miR-1915-3p (Fig. 3E) and miR-941 (Fig. 3G) levels in patients with PU was similar with the controls, and miR-194-3p (Fig. 3B), miR-491 (Fig. 3D), miR-1915-3p (Fig. 3F) and miR-941 (Fig. 3H) levels are comparable with each other among AA, AC and CC genotype groups. MMP9 mRNA level in patients with PU (Fig. 4A) was much higher than healthy controls, and also much higher in participants carrying AA genotype (Fig. 4B) than AC and CC genotypes, suggesting that interaction between miR-491 and MMP9 could be disrupted by the presence of the minor allele of the rs1056629 polymorphism.

Immunohistochemistry was carried out to determine MMP9 protein level among AA, AC and CC groups. As shown in Fig. 5A-C, MMP9 protein was highly expressed in AA group compared to that in AC and CC group, furthermore histology score in PU group was much higher in PU group than control group (Fig. 5D), and was also much higher in AA group than AC and CC groups (Fig. 5E), and histology score in AC and CC was similar with each other.

Real-time PCR and western blot analysis were performed to explore the effect of up- or downregulation of four miRNAs on the expression of MMP9. MMP9 levels in BJ fibroblast cells transfected with miR-194-3p, miR-491, miR-1915-3p or miR-941 mimic/inhibitor were measured. As shown in Fig. 6, only cells transfected with miR-491 mimic (Fig. 6B) showed evident decrease in MMP9 mRNA and protein compared with scramble control, while MMP9 mRNA and protein in BJ fibroblast cells transfected with miR-194-3p (Fig. 6A), miR-1915-3p (Fig. 6C) or miR-941 (Fig. 6D) mimic displayed no significant difference with scramble control. The MMP9 mRNA and protein levels in cells transfected with miR-491 inhibitor (Fig. 7B) was substantially improved compared with scramble control, and while MMP9 mRNA and protein levels in cells transfected with miR-194-3p (Fig. 7A), miR-1915-3p (Fig. 7C) or miR-941 (Fig. 7D) inhibitor were comparable with scramble control, verifying that miR-491 directly and negatively regulated MMP9 expression.