miRNA Profiling Workflow

Read more on activities performed.

1. Total RNA Isolation
   During sample homogenization or lysis, TRIZOL® Reagent maintains the integrity of the RNA while disrupting cells and dissolving cell components. Addition of chloroform followed by centrifugation, separates the solution into an aqueous phase and an organic phase. RNA remains exclusively in the aqueous phase. After transfer of the aqueous phase, the RNA is recovered by precipitation with isopropyl alcohol.  > Related products.
2. Amplification
   If necessary, amplify the enriched miRNA using t is added to the miRNA using poly A polymerase and an optimized reaction buffer. Then tailed miRNA is reverse-transcribed using SuperScript™ III RT, and purified and concentrated the resulting first-strand cDNA.
   Next, poly(dT) tail is added to the 3´ end of the first-strand product using terminal deoxynucleotidyl transferase, and synthesize and anneal a T7 promoter on the tailed cDNA using Klenow enzyme and a specially-designed T7 template oligo. Finally, an in vitro transcription reaction is performed with an overnight incubation to generate the amplified senseRNA. > Related products.
3. Labeling and Hybridization
   The NCode™ miRNA Rapid Labeling System tags the miRNAs in a simple 1-hour procedure and hybridizes them to the microarray. Using the Labeling System, a poly(A) tail is added to the miRNA using poly A polymerase and an optimized reaction buffer (this step if unnecessary if you are using amplified miRNA). Then a short, highly specific tag sequence is ligated to each tailed miRNA using a bridging oligo. Following a purification step, the tagged miRNA is hybridized to the microarray and incubated . Next the array is washed , hybridized with Alexa FluorR 3 and Alexa FluorR 5 capture reagents, washed again, and scaned using a standard microarray scanner. The capture reagents are comprised of DNA polymers, each with ~900 Alexa FluorR molecules bound to a sequence complementary to the ligated tags on the hybridized miRNAs. The high specificity of the binding sequence and high fluorescence of the dye molecules ensure maximum signal-tobackground ratios and strong signal correlations. > Related products.
4. Data Analysis
   Microarray signal intensities detected by the scanner are quantified by detection software. Signal intensities for each spot are calculated by subtracting local background and raw data are normalized and analyzed by using data analysis software. Learn more on data analysis methods typically used for normalization of 2-dye expression profiling microarray experiments.
5. Data Validation Using qRT-PCR
   Initially, the miRNAs are polyadenlyated using poly A polymerase and ATP. Following polyadenylation, SuperScript™ III RT and a specially-designed Universal RT Primer are used to synthesize cDNA from the tailed miRNA population. Subsequently, the first-strand cDNA is analyzed in qPCR using SYBR® Green or SYBR® GreenER™ detection reagents, a universal qPCR primer provided in the kit, and a forward primer designed by the user that targets the specific miRNA sequence of interest. > Related products.