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引用資料與參考文獻 (39)
Invitrogen™
Quant-iT™ RNA Assay Kits and Quant-iT RNA HS Reagent
Achieve highly selective and accurate quantification of high-abundance RNA samples with the fluorescent Quant-iT RNA Reagent and Assay Kits. These kits are highly selective for RNA over double-stranded DNA, and provide sufficient material for at least 2000 assays in a 96-well microplate format.
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變更視圖
| 產品號碼 | Quantity | Assay | Quantitation Range |
|---|---|---|---|
| Q33140 | 1 kit | RNA Quantitation | 5 to 100 ng |
| Q10213 | 1,000 assays | RNA Quantitation, BR | 20 to 1000 ng |
| Q33225 | 1000 assays | RNA Quantitation, ext range | 200 to 10,000 ng |
| Q32884 | 1 mL | RNA Quantitation, HS | 5 to 100 ng |
產品號碼 Q33140
價格 (TWD)
17,010.00
온라인 행사
Ends: 31-Dec-2025
24,300.00您節省 7,290.00 (30%)
Each
Quantity:
1 kit
Assay:
RNA Quantitation
Quantitation Range:
5 to 100 ng
價格 (TWD)
17,010.00
온라인 행사
Ends: 31-Dec-2025
24,300.00您節省 7,290.00 (30%)
Each
Enable easy and accurate RNA quantitation with the Quant-iT RNA Assay Kit, which is also available in broad range (BR) and extended range (XR) configurations, as well as a stand-alone high sensitivity (HS) reagent. These Quant-iT RNA quantification kits are highly selective for RNA over dsDNA and can be used to generate fluorescence-based linear detection ranges of RNA.
Quant-iT RNA Reagent and Assay Kit
The Quant-iT RNA Reagent and Assay Kit makes RNA quantification easy and accurate. The kit provides concentrated assay reagent, dilution buffer, and pre-diluted RNA standards. The assay is highly selective for RNA over double-stranded DNA, and provides a dynamic range of 5-100 ng of RNA.
Quant-iT RNA BR (Broad Range) Assay Kit
The Quant-iT RNA BR (Broad Range) Assay Kit provides an accurate and selective method for quantification of high-abundance RNA samples. While the original Quant-iT RNA kit has great sensitivity, the Quant-iT RNA Broad Range kit is ideal for microarray samples where the concentration of RNA is higher. The assay is highly selective for RNA over double-stranded DNA, and provides a dynamic range of 20-1000 ng of RNA.
Quant-iT RNA XR (Extended Range) Assay Kit
The Quant-iT RNA XR (Extended Range) Assay Kit provides an accurate and selective method for the quantification of high-abundance RNA samples. The assay is highly selective for RNA and does not quantitate DNA, protein, or free nucleotides. The assay kit is designed to be accurate for initial RNA sample concentrations of 10 ng/μL to 10,000 ng/μL depending on sample volume, providing a linear detection range of 200–10,000 ng.
For each assay, simply dilute the reagent using the buffer provided, add the sample (any volume between 1 μL and 20 μL is acceptable), and read the concentration using a fluorescence-based microplate reader. Common contaminants, such as salts, free nucleotides, solvents, detergents, and protein, are well tolerated.
The Quant-iT RNA Reagent and Assay Kit makes RNA quantification easy and accurate. The kit provides concentrated assay reagent, dilution buffer, and pre-diluted RNA standards. The assay is highly selective for RNA over double-stranded DNA, and provides a dynamic range of 5-100 ng of RNA.
Quant-iT RNA BR (Broad Range) Assay Kit
The Quant-iT RNA BR (Broad Range) Assay Kit provides an accurate and selective method for quantification of high-abundance RNA samples. While the original Quant-iT RNA kit has great sensitivity, the Quant-iT RNA Broad Range kit is ideal for microarray samples where the concentration of RNA is higher. The assay is highly selective for RNA over double-stranded DNA, and provides a dynamic range of 20-1000 ng of RNA.
Quant-iT RNA XR (Extended Range) Assay Kit
The Quant-iT RNA XR (Extended Range) Assay Kit provides an accurate and selective method for the quantification of high-abundance RNA samples. The assay is highly selective for RNA and does not quantitate DNA, protein, or free nucleotides. The assay kit is designed to be accurate for initial RNA sample concentrations of 10 ng/μL to 10,000 ng/μL depending on sample volume, providing a linear detection range of 200–10,000 ng.
For each assay, simply dilute the reagent using the buffer provided, add the sample (any volume between 1 μL and 20 μL is acceptable), and read the concentration using a fluorescence-based microplate reader. Common contaminants, such as salts, free nucleotides, solvents, detergents, and protein, are well tolerated.
For Research Use Only. Not for use in diagnostic procedures.
規格
AssayRNA Quantitation
For Use With (Equipment)Microplate Reader
No. of Reactions1000 Reactions (200 μL Assay Volume)
Product LineQuant-iT
Quantitation Range5 to 100 ng
Quantity1 kit
Shipping ConditionRoom Temperature
Detection MethodFluorescence
Unit SizeEach
常見問答集 (常見問題)
Why am I getting negative fluorescence values with my Qubit Assays?
I have a Quant-iT RNA Assay Kit and want to use it with the Qubit Fluorometer. Can I?
Will these Quant-iT RNA kits work for siRNA or microRNA?
Can the Quant-iT RNA assay be used to quantitate RNA labeled with digoxigenin?
What are the linear ranges of the Quant-iT RNA kits?
引用資料與參考文獻 (39)
引用資料與參考文獻
Abstract
Development and validation of endogenous reference genes for expression profiling of medaka (Oryzias latipes) exposed to endocrine disrupting chemicals by quantitative real-time RT-PCR.
Journal:Toxicol Sci
PubMed ID:17093204
The quantitative real-time reverse transcription polymerase chain reaction (Q-RT-PCR) technique has been increasingly used in endocrine disrupting chemicals (EDCs) research. Usually, an appropriate endogenous control gene is critical for Q-RT-PCR to normalize the errors and sample-to-sample variations that occur in the course of tissue collection, RNA isolation, and RT-PCR. In
Corn oil supplementation to steers grazing endophyte-free tall fescue. II. Effects on longissimus muscle and subcutaneous adipose fatty acid composition and stearoyl-CoA desaturase activity and expression.
Journal:J Anim Sci
PubMed ID:17431049
'Eighteen steers were used to evaluate the effect of supplemental corn oil level to steers grazing endophyte-free tall fescue on fatty acid composition of LM, stearoyl CoA desaturase (SCD) activity and expression as well as cellularity in s.c. adipose. Corn oil was supplemented (g/kg of BW) at 0 (none), 0.75
No compensation in CD44 stem cell marker following BCL-2 suppression by antisense oligonucleotides.
Journal:In Vivo
PubMed ID:23422486
'Antisense oligonucleotides have previously been used to target regulatory proteins in prostate cancer models. We evaluated mono- and bispecific oligonucleotides which comparably suppressed expression of B-cell lymphoma-2 (BCL-2) in LNCaP cells. Cells compensated by suppressing caspase-3 (an apoptosis promoter), and enhancing the expression of androgen receptor and co-activating p300 and
Suppression of prolactin-induced signal transducer and activator of transcription 5b signaling and induction of suppressors of cytokine signaling messenger ribonucleic acid in the hypothalamic arcuate nucleus of the rat during late pregnancy and lactation.
Journal:Endocrinology
PubMed ID:16857756
'During late pregnancy and lactation, the tuberoinfundibular dopamine (TIDA) neurons that regulate prolactin secretion by negative feedback become less able to produce dopamine in response to prolactin, leading to hyperprolactinemia. Because prolactin-induced activation of dopamine synthesis in these neurons requires the Janus kinase/signal transducer and activator of transcription 5b (STAT5b)
Reduced myocilin expression in cultured monkey trabecular meshwork cells induced by a selective glucocorticoid receptor agonist: comparison with steroids.
Journal:Invest Ophthalmol Vis Sci
PubMed ID:19696178
'To assess in vitro myocilin (MYOC) expression in trabecular meshwork (TM) cells exposed to BOL-303242-X, a selective glucocorticoid receptor (GR) agonist (SEGRA), in comparison with dexamethasone (DEX), and prednisolone acetate (PA). After drug treatment of monkey TM cultures, MYOC protein in conditioned media (CM) was measured by Western blot and