Adolescent Idiopathic Scoliosis Clinical Trial
— IMIRSAOfficial title:
Identification and Characterization of Circulating microRNAs as Diagnostic Biomarkers in Adolescent Idiopathic Scoliosis
The aim of the present study is to evaluate the expression of a large panel of microRNAs, already known and validated in other ortopedic pathologies and bone metabolism, in the plasma of Adolescent Idiopathic Scoliosis (AIS) patients. The deregulated microRNAs identified will be then validated and computational analyzes will determine their potential involvement in the metabolism of bone and/or cartilage tissue in order to correlate the results obtained with the clinical data of the AIS patients. The investigators aimed to develop a microRNAs panel to further validate in a larger population of AIS patients in order to produce a device for the diagnosis and prognosis of Molecular-based AIS.
Status | Recruiting |
Enrollment | 30 |
Est. completion date | July 21, 2024 |
Est. primary completion date | August 31, 2022 |
Accepts healthy volunteers | Accepts Healthy Volunteers |
Gender | All |
Age group | 11 Years to 17 Years |
Eligibility | Inclusion Criteria: Cases: - Age between 11-17 years - Diagnosis of idiopathic scoliosis with a Cobb angle> 10 ° - Minimum follow-up of two years - Clinical data and radiological tests available and no surgical treatment prior to enrollment in the study Controls: - Age between 11-17 years - Healthy subjects not affected by orthopedic and oncological diseases Exclusion Criteria: - Severe cognitive impairment or psychiatric disorders - Patients with scoliosis due to secondary causes - Women of childbearing age must not be pregnant |
Country | Name | City | State |
---|---|---|---|
Italy | Dipartimento Rizzoli-Sicilia | Bagheria |
Lead Sponsor | Collaborator |
---|---|
Istituto Ortopedico Rizzoli |
Italy,
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Type | Measure | Description | Time frame | Safety issue |
---|---|---|---|---|
Primary | Isolation of circulating microRNAs from AIS patients and healthy controls | Plasma samples will be obtained from blood samples of 20 AIS patients and 10 healthy subjects, collected in commercially available anticoagulant-treated tubes and centrifuged for 15 minutes at 2,000 x g. Circulating microRNAs will be isolated from the plasma samples by using commercially available miRNA Plasma Purification kit, specifically designed for purify high-quality microRNAs from plasma samples. Quantification and quality control of the purified circulating microRNAs will be determined through micro-spectrophotometry and microfluidics-based platforms. | Within 24 hours of blood sampling | |
Primary | Expression profiling of circulating microRNAs from AIS patients and healthy controls | The differentially expressed circulating microRNAs between AIS patients and healthy controls will be screened through micro-array technology using commercially available custom array microRNA cards, developed for profiling hundreds of unique human mature microRNAs known to be present in serum/plasma samples. | Within 2 months of blood sampling | |
Secondary | Bioinformatics analysis of circulating microRNAs in AIS patients and healthy controls. | The analysis of microRNA profiling data will be carried out by considering the value of | log2 (HR) | = 1.5 as differential expression limit of microRNA between the two groups of patients considered (AIS and control). The microRNAs not expressed in any sample will be excluded from the analysis.
After data normalization, the differently expressed microRNAs will be analyzed with an analysis of hierarchical clusters. The TargetScan database (http://targetscan.org/) and the miRDB database (http://mirdb.org/miRDB/) will be used to predict the potential target genes of differentially expressed microRNAs. Target gene function analysis of differentially expressed miRNAs will be carried out on the Gene Ontology software (GO, http://meme.nbcr.net/meme/cgi-bin/gomo.cgi) and Kyoto Encyclopedia Genes and Genomes (KEGG, http: // www.genome .jp / kegg / expression) |
Within 3 months of blood sampling | |
Secondary | Functional role of the circulating microRNAs related to AIS | To validate the microRNAs differentially expressed in the AIS patients compared to the healthy controls, specific qRT-PCR assays will be conducted in human bone cell lines (e.g. human primary osteoblasts, osteoclast, mesenchymal stem cells and chondrocyte cells). The role of microRNAs deregulated will be investigated in osteogenic, osteoclastic and chondrocyte differentiation by loss-of-function and gain-of-function experiments, in human bone cell lines (e.g. Runx2, ALP, Coll1A, OPN, OCN; TRAP, NFATc1, MMP9, CTSK; Coll2A, Sox9, ACAN). Viability assay (e.g. WST1 assay); apoptosis assay will be also performed (e.g. Annexin V staining assay, Caspase 3/7 assay and TUNEL detection methods). | Within 6 months of blood sampling |
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