TaqMan miRNA Assays for let-7dgi [32 (link)], C7, amiR-RICE, mmu-miR146a, MIR2911, and MIR168a were obtained from Life Technologies (Carlsbad, CA). Total RNA isolated was used in each reverse transcription (RT) reaction, as previously described [14 (link)]. To quantify miRNA levels in Arabidopsis, plant shoot material was ground to a fine powder in liquid nitrogen and then 10–20 mg was subjected to RNA isolation using the miRNeasy kit; 50 fmol of synthetic C7 was spiked into the plant Qiazol lysate as an exogenous RNA control. qRT-PCR was performed using a Biorad CFX96 Real-Time PCR Detection System, and data were analyzed using Biorad CFX software. Delta-Delta-Ct method was used to calculate the relative levels of miRNAs. Absolute concentrations of miRNAs were calculated based on standard curves obtained from serial dilutions of synthetic miRNAs [14 (link)] (Additional file 1 : Figure S1).
Mir168a
Manufactured by Thermo Fisher Scientific
MIR168a is a microRNA (miRNA) that is part of the Thermo Fisher Scientific product line. MIRNAs are small, non-coding RNA molecules that play a role in gene expression regulation. The core function of MIR168a is to serve as a research tool for studying miRNA expression and function. Detailed information about the intended use or specific applications of MIR168a is not available.
Automatically generated - may contain errors
Lab products found in correlation
Cfx96 real time pcr detection system, by Bio-Rad (4 mentions)
Mir2911, by Thermo Fisher Scientific (3 mentions)
Mir161, by Thermo Fisher Scientific (3 mentions)
Mir 16, by Thermo Fisher Scientific (2 mentions)
Mirneasy kit, by Qiagen (2 mentions)
Mir156a, by Thermo Fisher Scientific (2 mentions)
Let 7a, by Thermo Fisher Scientific (1 mentions)
Pgem t easy vector, by Promega (1 mentions)
4 protocols using mir168a
1
Quantification of miRNA Levels in Arabidopsis
2
Quantification of Plant and Serum miRNAs
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Taqman microRNA Assays for let-7d,g,i22 (link), let-7a, miR-16, MIR161, MIR2911, MIR168a, and C7 were obtained from Life Technologies (Grand Island, NY). For serum samples, total RNA equivalent to 10 μL of sera was used in each RT reaction. Of the 10 μL RT product, 1 μL was used for each triplicated qPCR reaction. To quantify miRNA levels in the plants, 10–30 mg of fresh plant material were ground to a fine powder in liquid nitrogen and then subjected to RNA isolation using the miRNEASY kit (Qiagen, Valencia, CA); 1 pmole of synthetic artificial miRNA C7 was spiked into the plant Qiazol lysate as an exogenous RNA control. The quantification result was normalized to the weight of starting plant material. qRT-PCR was performed using a Biorad CFX96 Real-Time PCR Detection System, and data were analyzed using Biorad CFX software9 (link). The Delta-Delta-Ct method was used to calculate relative levels of miRNAs. Absolute concentrations of miRNAs were calculated based on standard curves obtained from serial dilutions of synthetic miRNAs. The quantification Ct values all fall in the linear range of taqman assays as determined by the synthetic microRNA standards.
3
Quantitative Analysis of miRNA Expression
4
Quantification of Plant and Exosomal miRNAs
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Taqman microRNA Assays for let-7dgi [24 (link)], miR-16, MIR161, MIR2911, MIR156a, MIR168a and artificial miRNA C7 were obtained from Life Technologies. Total RNA equivalent to 10 μL of sera or 8 μL of urine were used in each reverse transcription (RT) reaction. Of the 10 μL RT product, 0.5 μL was used for each triplicated quantitative polymerase chain reaction (PCR). To quantify miRNA levels in herbs and flowers, 10 mg of dried plant material were ground to fine powder in liquid nitrogen and then subjected to RNA isolation using the miRNEASY kit (Qiagen); 1 pmol of synthetic MIR161 was spiked into the plant Qiazol lysate as an exogenous RNA control. qRT-PCR was performed using a Biorad CFX96 Real-Time PCR Detection System, and data were analyzed using Biorad CFX software. Delta-Delta-Ct method was used to calculate relative levels of miRNAs. Absolute concentrations of miRNAs were calculated based on standard curves obtained from serial dilutions of synthetic miRNAs. To verify the fidelity of Taqman microRNA assay kit for MIR2911, the qPCR product was agarose gel-purified and subcloned into pGEM-T Easy vector (Promega) and sequenced [25 (link)].
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