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Description:
Procedures such as cDNA synthesis, expression profiling, and others, require separation of mRNA from the vastly more abundant rRNA and tRNA. The GenElute mRNA Kits provide convenient procedures for isolating polyadenylated mRNA from previously prepared total RNA, or directly from mammalian cells and tissues.
For direct mRNA preparation, cells or tissues are disrupted with SDS/proteinase K digestion to release RNA and eliminate RNases. Both kit types use oligo dT30 covalently linked to 1 µm polystyrene beads to capture polyadenylated mRNA by hybridization. The polystyrene beads remain suspended during hybridization, eliminating the need for mixing or rocking, as is common for cellulose or magnetic particles. Polystyrene was also chosen because oligo (dT) polystyrene beads yield cleaner mRNA with fewer stringent washing steps than does the more commonly used oligo (dT) cellulose (2 or 3 wash steps versus 10 or more). With the GenElute kits, mRNA-bead complexes are washed on a microcentrifuge spin filter, and eluted into 10 mM Tris-HCl, pH 7.5. mRNA prepared with either kit is suitable for a variety of downstream applications such as Northern Blotting (Figure 4), Expression Array or Chip Hybridizations, and cDNA Synthesis and Library Construction. |
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Features and Benefits
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Fast
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Prep time is 40 minutes for poly A+ mRNA from total RNA or 60 minutes directly from cells and tissues.
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Convenient
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mRNA captured on polystyrene beads in 10 minutes, with no mixing or rocking. Beads washed on microcentrifuge spin filters.
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Yield
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Higher than all competing products.
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GenElute mRNA From Total RNA Kits
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Product Code
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Name
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Purifications per Kit
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Capacity
(µg Total RNA)
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Technical Manual .pdf
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Short Protocols .pdf
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GenElute mRNA Miniprep Kit
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10
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5-500
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GenElute mRNA Miniprep Kit
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70
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5-500
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GenElute Direct mRNA Kits
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Product Code
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Name
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Purifications per Kit
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Capacity
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Technical Manual .pdf
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Short Protocols .pdf
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GenElute Direct
mRNA Miniprep Kit
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10
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up to 107 up to 50mg
cells tissues
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GenElute Direct
mRNA Miniprep Kit
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70
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up to 107 up to 50mg
cells tissues
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Kit Contents
GenElute mRNA From Total RNA Kits
- Water, Molecular Biology Grade
- 2x Binding Solution
- Oligo (dT) Polystyrene Beads
- Wash Solution
- Elution Solution
- Spin Columns with Tubes
- Collection Tubes
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GenElute Direct mRNA Kits
Lysis Solution
- Proteinase K and Hydration Reagent
- 5 M NaCl
- Oligo (dT) Polystyrene Beads
- Wash Solutions 1 & 2
- Elution Solution
- Filtration Columns with Tubes
- Spin Columns with Tubes
- Collection Tubes
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Preparation Time Comparison
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Figure 1. Comparison of the preparation time, to isolate mRNA from total RNA or direct from cells or tissues, using GenElute mRNA Miniprep Kit and other commercially available kits. Each kit was prepared according to the procedure supplied by the vendor.
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RNA Yield
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Figure 2. Total RNA was prepared from Hek293 cells by a silica-binding method, using TriReagent®. mRNA was subsequently prepared from total RNA preparations using commercially available kits, following the procedures supplied by each vendor. RNA yield was measured using the RiboGreenTM RNA Quantitation Kit (Molecular Probes).
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Specific mRNA yield
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Figure 3. mRNA was prepared from total RNA as in Figure 2, and twenty percent of each preparation was analyzed by Northern blot hybridization with 32P-labeled probes. Hybridization to human HGPRT, human p53, and mouse p53 mRNAs were quantified with a Perkin Elmer Instant Imager.
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mRNA is suitable for Northern Blots
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Figure 4.
Northern blot comparison of mRNA prepared with GenElute mRNA
kits from other suppliers.
Duplicate mRNA samples were prepared from 5 x 106 Hek293
cells (top left panels) or 25-35 mg mouse liver (top right
panels) with Sigma's GenElute Direct mRNA Miniprep Kit (S)
or with another commercially available direct mRNA miniprep kit (A,
D, I, P, & Q). An optional release and rebind procedure (described
in the Manual) was
included for preparation S+: RNA was hybrid-captured onto oligo
(dT) beads, released into fresh lysis solution, and re-captured onto
the same beads before washing and eluting mRNA. The release and rebinding
steps were omitted for S- & Sx2 preparations. Sx2
preparations were repurified after the final elution with fresh oligo
(dT) beads (as described in the Manual)
. Equal portions of each mRNA preparation, equal to the amount from
1 x 106 cells or 10 mg liver, were evaluated by Northern
blot hybridization with 32P-labeled RNA probes
for p53, hypoxanthine-guanine phosphoribosyl transferase (HGPRT),
c-myc, and/or glyceraldehyde 3-phosphate dehydrogenase (GAPDH) mRNA.
For the bottom panels, total RNA was first prepared from Hek293
cells and from mouse liver. Duplicate mRNA samples were then prepared
from 100 µg of these total RNA preparations with Sigma's GenElute
mRNA Miniprep Kit (S) or with another commercially available mRNA
miniprep kit (Q, A, I, P, D). Samples Sx2 were repurified after elution.
Twenty percent of each preparation was evaluated by Northern blot
as above. In lanes T, 5 and 2 µg of the original total RNA from
cells or 10 and 5 µg of total RNA from liver were analyzed for
comparison. |
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