All RNA was isolated using RNeasy Plus Mini Kit (QIAGEN). RT-qPCR was performed using Brilliant II QRT-PCR SYBR® Green Low ROX Master Mix (Agilent Technologies) on an Applied Biosytems QuantStudio 6 Flex Real-Time PCR system using the indicated primers. Expression was normalized to Beta-actin (mouse) or GAPDH (human). Primer sequences are listed in Table S4 . Significance calculated by t test, error bars show standard error of the mean.
Brilliant 2 qrt pcr sybr green low rox master mix
Manufactured by Agilent Technologies
Sourced in United States
The Brilliant II QRT-PCR SYBR® Green Low ROX Master Mix is a reagent used for quantitative reverse transcription polymerase chain reaction (qRT-PCR) assays. It contains SYBR® Green dye for detection of double-stranded DNA amplification.
Automatically generated - may contain errors
Lab products found in correlation
Rneasy plus mini kit, by Qiagen (2 mentions)
Purelink genomic dna mini kit, by Thermo Fisher Scientific (2 mentions)
Purelink viral rna mini kit, by Thermo Fisher Scientific (2 mentions)
Mx3000p machine, by Agilent Technologies (1 mentions)
Brilliant 2 sybr green qrt pcr low rox master mix system, by Agilent Technologies (1 mentions)
Mx3000p quantitative pcr system, by Agilent Technologies (1 mentions)
6 protocols using brilliant 2 qrt pcr sybr green low rox master mix
1
RNA Expression Analysis by RT-qPCR
2
Quantifying Dino Gene Expression in Murine Spleens
Check if the same lab product or an alternative is used in the 5 most similar protocols
+ Expand
Splenic genomic DNA was prepared from 3-month-old Dino+/+, Dino+/− and Dino−/− (n = 3, 2 male and 1 female per genotype), and Dino+/−-Eμ-myc tumor bearing spleens dissected at time of death (Purelink Genomic DNA Mini Kit, Invitrogen). Q-PCR was carried out using primers specific to the endogenous Dino locus and EGFP (mutant allele, See Table S4 ), normalizing to L32 as a control (Brilliant II QRT-PCR SYBR® Green Low ROX Master Mix (Agilent Technologies), QuantStudio 6 Flex Real-Time PCR system (Applied Biosytems)). The relative abundance of Dino and EGFP in tumors is shown normalized to Dino+/− spleen.
3
Quantifying Dino Gene Expression in Murine Spleens
4
RNA Expression Analysis by RT-qPCR
Check if the same lab product or an alternative is used in the 5 most similar protocols
+ Expand
All RNA was isolated using RNeasy Plus Mini Kit (QIAGEN). RT-qPCR was performed using Brilliant II QRT-PCR SYBR® Green Low ROX Master Mix (Agilent Technologies) on an Applied Biosytems QuantStudio 6 Flex Real-Time PCR system using the indicated primers. Expression was normalized to Beta-actin (mouse) or GAPDH (human). Primer sequences are listed in Table S4 . Significance calculated by t test, error bars show standard error of the mean.
5
Dengue Virus RNA Detection and Serotyping
Check if the same lab product or an alternative is used in the 5 most similar protocols
+ Expand
Viral RNA was extracted from 200 μL of serum sample using the PureLink Viral RNA Mini Kit (Life Technologies, USA) according to the instructions from the manufacturer and immediately subjected to real-time qRT‒PCR. Real-time qRT‒PCR was performed with a Brilliant II SYBR Green qRT‒PCR Low ROX Master Mix system (Agilent, USA). In brief, a 25 μL mixture containing 5 μL of sample RNA, 0.25 μM forward and reverse DENV detecting or molecular-typing primers each, 2 × Brilliant II SYBR Green qRT‒PCR Low ROX Master Mix, RT/RNase Block Enzyme Mixture and RNase-free water was assayed in an Mx3000P machine (Agilent, USA). Dengue-specific primers for DENV RNA detection were DN-F: CAA TAT GCT GAA ACG CGA GAG AAA and DN-R: CCC CAT CTA TTC AGA ATC CCT GCT. Serotype-specific primers for molecular serotyping were DN-F: CAA TAT GCT GAA ACG CGA GAG AAA, D1-R CGC TCC ATA CAT CTT GAA TGA G, D2-R: AAG ACA TTG ATG GCT TTT GA, D3-R: AAG ACG TAA ATA GCC CCC GAC and D4-R: AGG ACT CGC AAA AAC GTG ATG AAT. The criteria of a positive control were a threshold cycle (Ct) value ≤ 30 and a Tm ≥ 79 °C, while a negative control had a Ct value ≥ 40 and a Tm < 79 °C. For the samples, a Ct value of ≤ 30 or a Tm ≥ 79 °C was considered positive [17 (link)].
6
Dengue Virus Detection by qRT-PCR
Check if the same lab product or an alternative is used in the 5 most similar protocols
+ Expand
Viral RNAs were extracted from 200 μl of the cell culture supernatants or serum samples using the PureLink® Viral RNA Mini Kit (Life Technologies; USA) according to the manufacturer’s instructions and stored at -80°C. Real-time qRT-PCR was performed using a Mx3000P quantitative PCR system (Agilent/Stratagene, USA). The samples were assayed in 25-μl reaction mixtures containing 5 μl of the sample RNA and 0.2 μM forward and reverse primers using the Brilliant II SYBR Green QRT-PCR Low ROX Master Mix and RT/RNase Block Enzyme Mixture (Agilent/Stratagene, USA). The primer sequences applied for detecting and typing the dengue viruses were published previously [10 (link)]. The thermal profile used for the one-step SYBR Green-based real-time qRT-PCR assay and the melting curve analysis were based on previously described information with minor modifications [10 (link)], and amplification plots and Tm values were routinely analyzed to verify the specificity of the amplicons.
About PubCompare
Our mission is to provide scientists with the largest repository of trustworthy protocols and intelligent analytical tools, thereby offering them extensive information to design robust protocols aimed at minimizing the risk of failures.
We believe that the most crucial aspect is to grant scientists access to a wide range of reliable sources and new useful tools that surpass human capabilities.
However, we trust in allowing scientists to determine how to construct their own protocols based on this information, as they are the experts in their field.
Ready to get started?
Sign up for free.
Registration takes 20 seconds.
Available from any computer
No download required
Revolutionizing how scientists
search and build protocols!