Expresión de miRNAs en orina como herramienta de diagnóstico y pronóstico en cáncer de próstata / Expression of urine miRNAs as a diagnostic and prognostic tool in prostate cancer

Resumen Introducción: El cáncer de próstata es la principal causa de muerte por cáncer en México, el diagnóstico inicial se hace mediante la medición del antígeno prostático específico y el tacto rectal de la próstata. Sin embargo, hay limitaciones que incluye la capacidad para distinguir con precisión los pacientes con y sin cáncer y aquellos que presentan una forma agresiva de la enfermedad. Los microRNAs se encuentran alterados en el tejido prostático canceroso, incluyendo aquellos casos fármaco resistentes. Los miRNAs son reguladores de la expresión génica y se encuentran involucrados en diversos procesos patológicos. Se ha demostrado que estas moléculas son detectables en orina. Objetivo: Esta revisión presenta la información sobre cuáles son los miRNAs reportados en orina como posibles marcadores para el diagnóstico, pronóstico y respuesta a la terapia en cáncer de próstata. Resultados: De la búsqueda realizada en la bibliografía, se encontraron 13 miRNAs en los diferentes estudios, miR-19a, miR-19b, miR-21, miR-148a, miR-375, miR-125b-5p, miR-151-5p, miR-141, miR-200b, miR-221, miR-107, miR-26b-5p, miR-205-5p. Teniendo algunos miRNAs como miR-375, miR-21, miR-141 encontrados en varios estudios. Limitaciones del estudio o implicaciones: Se puede concluir es factible obtener la medición por métodos no invasivos de miRNAs en pacientes con cáncer de próstata. Originalidad o valor: Es un estudio de revisión respecto a los miRNAs obtenidos en muestras de orina en pacientes con cáncer de próstata.

Abstract Introduction: Prostate cancer is the leading cause of cancer death in Mexico, the initial diagnosis is made by measuring the Prostate Specific Antigen and the digital rectal examination of the prostate. However, there are limitations including the ability to accurately distinguish patients with and without cancer and those with an aggressive form of the disease. MicroRNAs are altered in cancerous prostate tissue, including drug-resistant cases. MiRNAs are regulators of gene expression and are involved in various pathological processes. These molecules have been shown to be detectable in urine. Objective: This review presents the information on which are the miRNAs reported in urine as possible markers for the diagnosis, prognosis and response to therapy in prostate cancer. Results: From the literature search, 13 miRNAs were found in the different studies, miR-19a, miR-19b, miR-21, miR-148a, miR-375, miR-125b-5p, miR-151-5p , miR-141, miR-200b, miR-221, miR-107, miR-26b-5p, miR-205-5p. Having some miRNAs like miR-375, miR-21, miR-141 found in various studies. Limitations of the study or implications: It can be concluded that it is feasible to obtain the measurement of miRNAs by non-invasive methods in patients with prostate cancer. Originality or value: It is a review study regarding miRNAs obtained in urine samples in patients with prostate cancer.

Nosocomial transmission of extensively drug resistant Acinetobacter baumannii strains in a tertiary level hospital.

Acinetobacter baumannii is an opportunistic infectious agent that affects primarily immunocompromised individuals. A. baumannii is highly prevalent in hospital settings being commonly associated with nosocomial transmission and drug resistance. Here, we report the identification and genetic characterization of A. baumannii strains among patients in a tertiary level hospital in Mexico. Whole genome sequencing analysis was performed to establish their genetic relationship and drug resistance mutations profile. Ten genetically different, extensively drug resistant strains were identified circulating among seven wards. The genetic profiles showed resistance primarily against aminoglycosides and beta-lactam antibiotics. Importantly, no mutants conferring resistance to colistin were observed. The results highlight the importance of implementing robust classification schemes for advanced genetic characterization of A. baumannii clinical isolates and simultaneous detection of drug resistance markers for adequate patient's management in clinical settings.

Evaluation of the effect of heat damage on DNA extracted from the dental pulp of restored teeth.

We evaluate structural damage effects of heat on DNA obtained from the dental pulp of restored premolars. We studied three groups (A, B and C) each group comprised twenty premolars extracted from five patients. Three of the four premolars of each donator were restored with different materials: amalgam, glass ionomer and resin, and one unrestored premolar was used as control. The group A was not exposed to heat, while B and C groups were exposed to 100 °C and 300 °C, respectively. The DNA damage was evaluated as percentage of genotyping of 15 Short Tandem Repeats (STRs) and amelogenin and by Fourier-transform infrared spectroscopy (FTIR). The results showed 100% genotyping in all unheated premolars; however, the increase in heat decreased genotyping percentage due to DNA degradation. The amplifications from the premolars restored with glass ionomer and those unrestored were less affected, amplifying by approximately 80% at 300 °C. FTIR revealed that DNA structural damage occurred in the phosphate region, and changes in ribose were also shown; in addition, we detected presence of ß- three-calcium-phosphate (ß - TCP) due to heat treatment. Moreover, the phosphate region of DNA was a good indicator of DNA integrity related to the ratio of 1230/1085 cm-1 in the second derivative (asymmetric/symmetric PO2), which was major in premolars restored with glass ionomer heated at 100 °C, and this ratio is related to less DNA alterations and better genotyping; however this changes only were detected at 100 °C, suggesting that dental restoration with this material only protects dental pulp at temperatures below 300 °C.

Mitochondrial T16189C Polymorphism Is Associated with Metabolic Syndrome in the Mexican Population.

Genetic factors, such as the mitochondrial DNA (mtDNA) T16189C polymorphism, have been associated with metabolic syndrome (MetS), but this association has not been studied in Mexico to date. The aim of the present study was to determine whether this polymorphism contributes to MetS in the Mexican population. We recruited 100 unrelated volunteer subjects who were divided into 2 groups: with MetS (MetS group) and without MetS (control group). All subjects were genotyped for the mtDNA T16189C polymorphism by polymerase chain reaction and sequencing. The mitochondrial T16189C polymorphism was detected in 24 (24%) of 100 subjects analyzed. The frequency of the mtDNA T16189C polymorphism was higher in the MetS group with 21 (32.3%) of 65 testing positive compared to 3 (8.5%) of 35 in the control group, indicating that this polymorphism is a probable risk factor for MetS in the Mexican population (odds ratio 5.0909, 95% CI 1.3977-18.5424, P = 0.0136). Our results may contribute to early diagnosis of MetS, which is essential for establishing changes in early stages of the disease to avoid further complications and pathologies, thereby preventing the development of type 2 diabetes and cardiovascular disease in Mexico.