Your search keyword '"Sabaliauskaitė, Rasa"' showing total 2 results

1. Urine Molecular Biomarkers for Detection and Follow-Up of Small Renal Masses.

Author

Žalimas, Algirdas, Kubiliūtė, Raimonda, Žukauskaitė, Kristina, Sabaliauskaitė, Rasa, Trakymas, Mantas, Letautienė, Simona, Kaubrienė, Edita Mišeikytė, Ušinskienė, Jurgita, Ulys, Albertas, and Jarmalaitė, Sonata

Subjects

URINE, RENAL cell carcinoma, EARLY diagnosis, WATCHFUL waiting, BIOMARKERS, POLYMERASE chain reaction, DNA methylation

Abstract

Active surveillance (AS) is the best strategy for small renal masses (SRMs) management; however, reliable methods for early detection and disease aggressiveness prediction are urgently needed. The aim of the present study was to validate DNA methylation biomarkers for non-invasive SRM detection and prognosis. The levels of methylated genes TFAP2B, TAC1, PCDH8, ZNF677, FLRT2, and FBN2 were evaluated in 165 serial urine samples prospectively collected from 39 patients diagnosed with SRM, specifically renal cell carcinoma (RCC), before and during the AS via quantitative methylation-specific polymerase chain reaction. Voided urine samples from 92 asymptomatic volunteers were used as the control. Significantly higher methylated TFAP2B, TAC1, PCDH8, ZNF677, and FLRT2 levels and/or frequencies were detected in SRM patients' urine samples as compared to the control. The highest diagnostic power (AUC = 0.74) was observed for the four biomarkers panel with 92% sensitivity and 52% specificity. Methylated PCDH8 level positively correlated with SRM size at diagnosis, while TFAP2B had the opposite effect and was related to SRM progression. To sum up, SRMs contribute significantly to the amount of methylated DNA detectable in urine, which might be used for very early RCC detection. Moreover, PCDH8 and TFAP2B methylation have the potential to be prognostic biomarkers for SRMs. [ABSTRACT FROM AUTHOR]

Published

2022

2. The Role of TSHR, PTEN and RASSF1A Promoters' Methylation Status for Non-Invasive Detection of Papillary Thyroid Carcinoma.

Author

Klimaitė, Raimonda, Kazokaitė, Mintautė, Kondrotienė, Aistė, Daukšienė, Dalia, Sabaliauskaitė, Rasa, Žukauskaitė, Kristina, Žilaitienė, Birutė, Jarmalaitė, Sonata, and Daukša, Albertas

Subjects

THYROID cancer, PAPILLARY carcinoma, METHYLATION, DNA methylation, LYMPHATIC metastasis, POLYMERASE chain reaction, THYROIDECTOMY

Abstract

Aim: We investigated whether a difference exists between TSHR, PTEN and RASSF1A methylation status in plasma of subjects with papillary thyroid cancer (PTC). Methods: Peripheral blood samples were collected from 68 patients with PTC and 86 healthy controls (HC). Thyroid cancer tissue and corresponding adjacent normal tissue methylation levels were analyzed. DNA methylation level changes in TSHR, PTEN and RASSF1A genes were analyzed by quantitative methylation-sensitive polymerase chain reaction. Results: We observed that the methylation level of TSHR was significantly higher in the thyroid cancer tissue compared to adjacent normal tissue (p = 0.040). TSHR methylation levels in the PTC group plasma samples were significantly higher compared to HC (p = 0.022). After surgery, PTC plasma samples showed lower TSHR and PTEN methylation levels compared to the levels before surgery (p = 0.003, p = 0.031, respectively). The TSHR methylation level was significantly higher in PTC with larger tumor size (>2 cm) (p < 0.001), and lymph node metastases (p = 0.01), lymphovascular invasion (p = 0.02) and multifocality (p = 0.013) 0ROC analysis revealed that the TSHR methylation level provides high accuracy in distinguishing PTC from HC (p = 0.022, AUC of 0.616). Conclusion: TSHR methylation in peripheral blood samples is expected to be a sensitive and specific minimally invasive tool for the diagnosis of PTC, especially in combination with other diagnostic means. [ABSTRACT FROM AUTHOR]

Published

2022