콘텐츠로 건너뛰기
Merck
모든 사진(4)

문서

12033674001

Roche

High Pure RNA Tissue Kit

sufficient for 50 isolation(s), suitable for RT-PCR, suitable for Northern blotting

동의어(들):

RNA purification

로그인조직 및 계약 가격 보기
모든 사진(4)

About This Item

UNSPSC 코드:
41105500

사용

sufficient for 50 isolation(s)

Quality Level

100

제조업체/상표

Roche

포장

kit of for 50 isolations

기술

Northern blotting: suitable
RT-PCR: suitable

관련 카테고리

일반 설명

The High Pure RNA Tissue Kit is designed for the purification of total, intact RNA from tissue samples, free of any contaminating DNA. Low to medium throughput RNA isolation. Nucleic acids bind to the surface of the glass fleece in the presence of a chaotropic salt (guanidine HCl). This allows the High Pure Filter Tube to specifically immobilize nucleic acids (both DNA and RNA) while they are freed of contaminants. For RNA isolation, the binding conditions can be optimized to ensure immobilization of all the RNA. High pure RNA isolation kit can rapidly isolate intact total RNA from a broad range of research sample materials, including cultured cells, mammalian blood, white blood cells (WBCs), yeast, and bacteria. It rapidly isolates total RNA from mammalian tissues such as mouse liver, spleen, lung, and heart.

Capacity: The High Pure Spin Filter Tubes hold up to 700 μL sample volume.
Sample Material: Solid tissue (e.g., mouse liver, spleen, lung, heart): 1 - 25 mg.

Note: Sample size depends on the method used to prepare the tissue; larger samples (>10 mg) should be processed via rotor-stator homogenization.

애플리케이션

High Pure RNA Tissue Kit has been used:
  • to extract total RNA from human cells for cDNA library generation
  • to extract total RNA from cultured cells for real time PCR analysis
  • to extract total RNAs from rat hippocampi
  • to purify total RNA from cultured cells and human spinal cord
  • to isolate total RNA of tissues collected from ventricle walls


The isolated RNA can be used in many downstream applications:,
  • Northern blotting
  • RACE
  • primer extension
  • differential display
  • RNase protection assay
  • in vitro translation

특징 및 장점

  • Prepare RNA samples in approximately 30 minutes.
  • Obtain concentrated RNA that is suitable for downstream applications.
  • Minimize RNA loss with a kit that removes contaminants without precipitation or other handling steps that degrade RNA.
  • Eliminate the use of hazardous organic compounds such as cesium chloride, phenol, chloroform, and ethidium bromide.

성분

  • Lysis/Binding Buffer
  • DNase I, lyophilizate
  • DNase Incubation Buffer
  • Wash Buffer I
  • Wash Buffer II
  • Elution Buffer
  • High Pure Spin Filter Tubes (containing glass fiber fleece)
  • Collection Tubes

품질

  • Tissue is disrupted and homogenized in Lysis/Binding Buffer and purified as described.
  • RNA yield is determined by measuring the optical density at 260 nm.
  • Integrity and size distribution are examined by the banding pattern of ribosomal RNA in a denaturing agarose gel.
  • 10 μL of the RNA eluate is used in first strand synthesis with reverse transcriptase M-MuLV and p(dT)15 as primer. In the following PCR, accomplished using the Expand High Fidelity PCR System and specific primers for glycerinaldehyde 3-phosphate dehydrogenase (GAPDH), the expected amplification product of 983 bp is obtained.
  • Absence of contaminating DNA is examined by a PCR without a preceding RT reaction; no amplification product is obtained.

제조 메모

Tissue samples are disrupted and homogenized in the presence of a chaotropic salt (guanidine HCL) that inactivates RNases. The homogenate is then applied to the glass fiber fleece in a High Pure Spin Filter Tube. Under the buffer conditions used in the procedure, all nucleic acids bind to the glass fiber fleece, while contaminating substances (salts, proteins, and other cellular contaminants) do not. DNA in the preparation is digested with DNase I directly on the filter. Brief wash-and-spin steps readily remove the digested DNA fragments and other cellular contaminants. The remaining purified RNA is then eluted in a small volume of low-salt buffer.

기타 정보

High Pure Technology and Silica Adsorption Kits
For life science research only. Not for use in diagnostic procedures.
Figure 1: Comparison of different homogenization procedures. Mouse liver was homogenized using various procedures. Total RNA was purified from each of these homogenates with the High Pure RNA Tissue Kit. Aliquots of the isolated RNA were reverse transcribed with primers specific for a region of the GADH mRNA. cDNA products were analyzed via gel electrophoresis.

Lane 1: Homogenization: Ultra Turrax; yield: 1.9 μg/mg tissue; A 260/ A 280 : 2.0
Lane 2: Homogenization: motor-driven, disposable plastic pestle; yield: 3 μg/mg tissue; A 260 /A 280 : 2.0
Lane 3: Homogenization: mortar and pestle, 20 G needle; yield: 1.5 μg/mg tissue; A 260 /A 280 : 2.0
Lane 4: Homogenization: manual disposable plastic pestle, 20 G needle; yield: 1.8 μg/mg tissue; A 260 /A 280 : 2.0
Lane 5: Homogenization: manual disposable plastic pestle; yield: 3.4 μg/mg tissue; A 260 /A 280 : 2.0
Lane 6: Homogenization: bead-vortex; yield: 3 μg/mg tissue; A 260 /A 280 : 2.0
Lane 7: Molecular weight marker

픽토그램

Exclamation markHealth hazard
GHS07,GHS08

신호어

Danger

유해 및 위험 성명서

H302 + H332,H315,H317,H319,H334

Hazard Classifications

Acute Tox. 4 - Acute Tox. 4 Oral - Eye Irrit. 2 - Resp. Sens. 1 - Skin Irrit. 2 Inhalation - Skin Sens. 1

Storage Class Code

12 - Non Combustible Liquids

WGK

WGK 1

Flash Point (°F)

does not flash

Flash Point (°C)

does not flash

시험 성적서(COA)

제품의 로트/배치 번호를 입력하여 시험 성적서(COA)을 검색하십시오. 로트 및 배치 번호는 제품 라벨에 있는 ‘로트’ 또는 ‘배치’라는 용어 뒤에서 찾을 수 있습니다.

이 제품을 이미 가지고 계십니까?

문서 라이브러리에서 최근에 구매한 제품에 대한 문서를 찾아보세요.

문서 라이브러리 방문

이미 열람한 고객

Slide 1 of 1

1 of 1

GenElute™ Mammalian Total RNA Miniprep Kit sufficient for 10 purifications

Sigma-Aldrich

RTN10

GenElute Mammalian Total RNA Miniprep Kit

Kamila Nowak et al.
Epigenetics, 6(8), 1012-1020 (2011-07-05)
The monoallelic expression of imprinted genes is controlled by epigenetic factors including DNA methylation and histone modifications. In mouse, the imprinted gene Gtl2 is associated with two differentially methylated regions: the IG-DMR, which serves as a gametic imprinting mark at
Yan Chen et al.
Artificial cells, nanomedicine, and biotechnology, 47(1), 1788-1796 (2019-05-08)
Ropivacaine is a commonly used local anaesthetic, but its side effects remain largely unknown. In the present study, we investigated the side effects of ropivacaine in human neuronal SH-5Y5Y cells. We show that 0.5% and 1% ropivacaine could cause fission-like
Hasan Şimşek et al.
Iranian journal of basic medical sciences, 19(2), 209-214 (2016-04-16)
Ischemia is described as organs and tissues are destitute of oxygen due to decreased arterial or venous blood flow. Many mechanisms play role in cell death happened as a consequence of a new blood flow is needed for both cell
Faezeh Vahdati Hassani et al.
Daru : journal of Faculty of Pharmacy, Tehran University of Medical Sciences, 22(1), 16-16 (2014-01-10)
Antidepressants have been shown to affect levels of brain-derived neurotrophic factor (BDNF) and VGF (non-acronymic) whose transcriptions are dependent on cAMP response element binding protein (CREB) in long term treatment. The aim of this study was to verify the subacute
LingJun Zhan et al.
TheScientificWorldJournal, 2012, 907095-907095 (2012-05-31)
The real-time PCR diagnostics for avian influenza virus H5N1 in tissue specimens are often suboptimal, since naturally occurring PCR inhibitors present in samples, or unanticipated match of primer to unsequenced species' genome. With the principal aim of optimizing the SYBR
모든 관련된 서류 보기

자사의 과학자팀은 생명 과학, 재료 과학, 화학 합성, 크로마토그래피, 분석 및 기타 많은 영역을 포함한 모든 과학 분야에 경험이 있습니다..

고객지원팀으로 연락바랍니다.