2016
DOI: 10.1177/0004563216671538
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Stabilization of circulating thyroglobulin mRNA transcripts in patients treated for differentiated thyroid carcinoma

Abstract: Background The clinical utility of serum thyroglobulin in the follow-up of patients with differentiated thyroid carcinoma may be compromised by the presence of endogenous antithyroglobulin antibodies. To prevent interference by antithyroglobulin antibodies several groups have developed real-time PCR-based assays for quantification of blood thyroglobulin mRNA levels. For accurate quantification of thyroglobulin mRNA in blood preanalytical factors must be recognized and controlled. In this study, we evaluate the… Show more

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Cited by 6 publications
(5 citation statements)
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“…However, no significant differences in RIN at 25 • C (p = 0.787) or 40 • C (p = 0.399) was found for tube types (Figure 1A). In agreement with previously published studies [9,16], these results demonstrated that RNA integrity is temperature-sensitive, and that both tube types produced low-quality RNA at increased storage times and temperatures. Nevertheless, our data suggest that Tempus ™ tubes may provide better RNA integrity (higher RIN values) under certain suboptimal tropical conditions compared to PAXgene ® tubes.…”
Section: The Highest Quality Rna Was Obtained Using Tempus ™ Blood Rn...supporting
confidence: 92%
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“…However, no significant differences in RIN at 25 • C (p = 0.787) or 40 • C (p = 0.399) was found for tube types (Figure 1A). In agreement with previously published studies [9,16], these results demonstrated that RNA integrity is temperature-sensitive, and that both tube types produced low-quality RNA at increased storage times and temperatures. Nevertheless, our data suggest that Tempus ™ tubes may provide better RNA integrity (higher RIN values) under certain suboptimal tropical conditions compared to PAXgene ® tubes.…”
Section: The Highest Quality Rna Was Obtained Using Tempus ™ Blood Rn...supporting
confidence: 92%
“…This ratio is decreased in the presence of residual phenol, salts, and carbohydrates that can affect the accuracy of downstream application and used as a secondary measurement for RNA purity [38]. Historically, low A260/A230 ratios are reportedly attributed to the high salt content of the elution buffers contained in PAXgene ® extraction kits [16,17,34,35] and as well as in Tempus ™ extraction kits [16,22,39].…”
Section: Discussionmentioning
confidence: 99%
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“…With respect to the purity of the RNA, the best results were obtained with Methodology C. Overall, 'very good' and comparable purity values were observed for Methodology A and Methodology C, in accordance with previous research [9,12,20]. However, we observed more unstable A 260 /A 230 ratios with Methodology A and especially for Methodology B than these previous studies.…”
Section: Discussionsupporting
confidence: 90%
“…The cfRNA was immediately isolated from 4 mL of the supernatant of the second centrifugation using the QIAsymphony ® DSP Virus/Pathogen Midi Kit in a QIAsymphony robot (Qiagen, Hilden, Germany), following the manufacturer's instructions. The maximum 24‐h interval between blood collection and RNA purification was decided based on a stability study performed in‐house (Table S3 ), which was in line with previous publications about RNA stability in K2‐EDTA tubes [ 22 , 23 , 24 , 25 ]. The automatic extraction procedure is based on magnetic particles and involves bind, wash, and elution steps.…”
Section: Methodsmentioning
confidence: 99%