R2101,   Direct-zol-96 MagBead RNA (2x96 preps) w/ TRI Reagent [Includes E1009 DNase I Set (250 U) w/ 10X Reaction Buffer (1 ml) x 4 & R2050-1-200 x 1– packaged separately]

R2101, Direct-zol-96 MagBead RNA (2x96 preps) w/ TRI Reagent [Includes E1009 DNase I Set (250 U) w/ 10X Reaction Buffer (1 ml) x 4 & R2050-1-200 x 1– packaged separately]

R2103,   Direct-zol-96 MagBead RNA (4x96 preps) w/ TRI Reagent  [Includes E1009 DNase I Set (250 U) w/ 10X Reaction Buffer (1 ml) x 8 & R2050-1-200 x 2 – packaged separately]

R2103, Direct-zol-96 MagBead RNA (4x96 preps) w/ TRI Reagent [Includes E1009 DNase I Set (250 U) w/ 10X Reaction Buffer (1 ml) x 8 & R2050-1-200 x 2 – packaged separately]

R2102, Direct-zol-96 MagBead RNA (4x96 preps) [Includes E1009 DNase I Set (250 U) w/ 10X Reaction Buffer (1 ml) x 8 – packaged separately]

7.794,50 RON

The Direct-zol™-96 MagBead RNA kit provides a high-throughput (96-well), magnetic bead-based isolation of high-quality RNA directly from samples in TRI Reagent® and similar. The extraction method inactivates viruses and other infectious agents. Total RNA including small/microRNAs (≥17 nt) are effectively isolated from a variety of sample sources (cells, tissues, biological liquids, etc.). The procedure is easy: simply add ethanol and MagBinding Beads to a sample in TRI Reagent®, wash and elute the RNA. No phase separation, precipitation, or post-purification steps are necessary. The result is broad range purification of small and large RNAs suitable for subsequent RNA-based methods including Next-Gen sequencing, RT-PCR, transcription profiling, hybridization, etc.

SKU
ZR_R2102
HIGHLIGHTS

  • Easy Handling: Bypass chloroform, phase separation and precipitation steps.
  • NGS-Ready: Ultra-pure RNA without phenol carryover. No DNA contamination (DNase I included).
  • Non-Biased: Complete RNA recovery without miRNA loss.
DESCRIPTION

 

The Direct-zol™-96 MagBead RNA kit provides a high-throughput (96-well), magnetic bead-based isolation of high-quality RNA directly from samples in TRI Reagent® and similar. The extraction method inactivates viruses and other infectious agents. Total RNA including small/microRNAs (≥17 nt) are effectively isolated from a variety of sample sources (cells, tissues, biological liquids, etc.). The procedure is easy: simply add ethanol and MagBinding Beads to a sample in TRI Reagent®, wash and elute the RNA. No phase separation, precipitation, or post-purification steps are necessary. The result is broad range purification of small and large RNAs suitable for subsequent RNA-based methods including Next-Gen sequencing, RT-PCR, transcription profiling, hybridization, etc.

Learn More

For automation scripts and support, email automation@zymoresearch.com

 

TECHNICAL SPECIFICATIONS

Compatibility TRIzol®, RNAzol®, QIAzol®, TriPure™, TriSure™ and all other acid-guanidinium-phenol based solutions can be used in place of TRI Reagent®.
Equipment Microcentrifuge, vortex, magstand
Sample Inactivation TRI Reagent® (provided with R2101, R2103, and R2105) inhibits RNase activity and inactivates viruses and other infectious agents.
Sample Source Any sample stored and preserved in TRI Reagent®, TRIzol® or similar (animal cells, tissue, bacteria, yeast, fecal, biological fluids, and in vitro processed RNA (e.g., transcription products, DNase-treated or labeled RNA)).
Size Range Total RNA ≥ 17 nt
Yield 10 µg RNA (binding capacity), ≥ 30 µl (elution volume)
Mai multe informatii
Price 6.550,00 RON (preturile sunt fara TVA)
Description
HIGHLIGHTS

  • Easy Handling: Bypass chloroform, phase separation and precipitation steps.
  • NGS-Ready: Ultra-pure RNA without phenol carryover. No DNA contamination (DNase I included).
  • Non-Biased: Complete RNA recovery without miRNA loss.
DESCRIPTION

 

The Direct-zol™-96 MagBead RNA kit provides a high-throughput (96-well), magnetic bead-based isolation of high-quality RNA directly from samples in TRI Reagent® and similar. The extraction method inactivates viruses and other infectious agents. Total RNA including small/microRNAs (≥17 nt) are effectively isolated from a variety of sample sources (cells, tissues, biological liquids, etc.). The procedure is easy: simply add ethanol and MagBinding Beads to a sample in TRI Reagent®, wash and elute the RNA. No phase separation, precipitation, or post-purification steps are necessary. The result is broad range purification of small and large RNAs suitable for subsequent RNA-based methods including Next-Gen sequencing, RT-PCR, transcription profiling, hybridization, etc.

Learn More

For automation scripts and support, email automation@zymoresearch.com

 

TECHNICAL SPECIFICATIONS

Compatibility TRIzol®, RNAzol®, QIAzol®, TriPure™, TriSure™ and all other acid-guanidinium-phenol based solutions can be used in place of TRI Reagent®.
Equipment Microcentrifuge, vortex, magstand
Sample Inactivation TRI Reagent® (provided with R2101, R2103, and R2105) inhibits RNase activity and inactivates viruses and other infectious agents.
Sample Source Any sample stored and preserved in TRI Reagent®, TRIzol® or similar (animal cells, tissue, bacteria, yeast, fecal, biological fluids, and in vitro processed RNA (e.g., transcription products, DNase-treated or labeled RNA)).
Size Range Total RNA ≥ 17 nt
Yield 10 µg RNA (binding capacity), ≥ 30 µl (elution volume)
Manufacturer Zymo Research

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