2024年2月26日发(作者:)

1. HOMOGENIZATION (see notes 1-3)

a. Tissues

TRIZOL®

Reagent

Cat. No. 15596-026

Store at 2 to 8°C.

Size: 100 ml

WARNING: Toxic in contact with skin and if swallowed. Causes burns. After

contact with skin, wash immediately with plenty of detergent and water. If you feel

unwell, seek medical advice (show label where possible). Phenol (108-95-2) and Other

Components (NJTSRN 80100437-5000p).

TRIZOL has demonstrated stability of 12 months when stored at room temperature. However, we

recommend storage at 2 to 8°C for optimal performance.

Description:

TRIZOL Reagent ( No.5,346,994) is a ready-to-use reagent for the isolation of total RNA

from cells and tissues. The reagent, a mono-phasic solution of phenol and guanidine isothiocyanate,

is an improvement to the single-step RNA isolation method developed by Chomczynski and Sacchi

(1). During sample homogenization or lysis, TRIZOL Reagent maintains the integrity of the RNA,

while disrupting cells and dissolving cell components. Addition of chloroform followed by

centrifugation, separates the solution into an aqueous phase and an organic phase. RNA remains

exclusively in the aqueous phase. After transfer of the aqueous phase, the RNA is recovered by

precipitation with isopropyl alcohol. After removal of the aqueous phase, the DNA and proteins in

the sample can be recovered by sequential precipitation (2). Precipitation with ethanol yields DNA

from the interphase, and an additional precipitation with isopropyl alcohol yields proteins from the

organic phase (2). Copurification of the DNA may be useful for normalizing RNA yields from

sample to sample.

This technique performs well with small quantities of tissue (50-100 mg) and cells (5 × 106), and

large quantities of tissue (≥1 g) and cells (>107), of human, animal, plant, or bacterial origin. The

simplicity of the TRIZOL Reagent method allows simultaneous processing of a large number of

samples. The entire procedure can be completed in one hour. Total RNA isolated by TRIZOL

Reagent is free of protein and DNA contamination. It can be used for Northern blot analysis, dot blot

hybridization, poly (A)+ selection, in vitro translation, RNase protection assay, and molecular

cloning. For use in the polymerase chain reaction (PCR*), treatment of the isolated RNA with

amplification grade DNase I (Cat. No. 18068) is recommended when the two primers lie within a

single exon.

TRIZOL Reagent facilitates isolation of a variety of RNA species of large or small molecular size.

For example, RNA isolated from rat liver, electrophoresed on an agarose gel, and stained with

ethidium bromide, shows discrete bands of high molecular weight RNA between 7 kb and 15 kb in

size, (composed of mRNA’s and hnRNA’s) two predominant ribosomal RNA bands at ~5 kb (28S)

and at ~2 kb (18S), and low molecular weight RNA between 0.1 and 0.3 kb (tRNA, 5S). The

isolated RNA has an A260/A280 ratio ≥1.8 when diluted into TE.

Precautions for Preventing RNase Contamination:

RNases can be introduced accidentally into the RNA preparation at any point in the isolation

procedure through improper technique. Because RNase activity is difficult to inhibit, it is essential

to prevent its introduction. The following guidelines should be observed when working with RNA.

Always wear disposable gloves. Skin often contains bacteria and molds that can contaminate

an RNA preparation and be a source of RNases. Practice good microbiological technique to

prevent microbial contamination.

Use sterile, disposable plasticware and automatic pipettes reserved for RNA work to prevent

cross-contamination with RNases from shared equipment. For example, a laboratory that is

using RNA probes will likely be using RNase A or T1 to reduce background on filters, and any

nondisposable items (such as automatic pipettes) can be rich sources of RNases.

In the presence of TRIZOL Reagent, RNA is protected from RNase contamination. Downstream

sample handling requires that nondisposable glassware or plasticware be RNase-free. Glass

items can be baked at 150°C for 4 hours, and plastic items can be soaked for 10 minutes in 0.5

M NaOH, rinsed thoroughly with water, and autoclaved.

Other Precautions:

Use of disposable tubes made of clear polypropylene is recommended when working with less

than 2-ml volumes of TRIZOL Reagent.

For larger volumes, use glass (Corex) or polypropylene tubes, and test to be sure that the tubes

can withstand 12,000 × g with TRIZOL Reagent and chloroform. Do not use tubes that leak or

crack.

Carefully equilibrate the weights of the tubes prior to centrifugation.

Glass tubes must be sealed with parafilm topped with a layer of foil, and polypropylene tubes

must be capped before centrifugation.

INSTRUCTIONS FOR RNA ISOLATION:

Caution: When working with TRIZOL Reagent use gloves and eye protection (shield, safety

goggles). Avoid contact with skin or clothing. Use in a chemical fume hood. Avoid breathing

vapor.

Homogenize tissue samples in 1 ml of TRIZOL Reagent per 50-100 mg of tissue using a

glass-Teflon® or power homogenizer (Polytron, or Tekmar's TISSUMIZER® or

equivalent). The sample volume should not exceed 10% of the volume of TRIZOL

Reagent used for homogenization.

b. Cells Grown in Monolayer

Lyse cells directly in a culture dish by adding 1 ml of TRIZOL Reagent to a 3.5 cm

diameter dish, and passing the cell lysate several times through a pipette. The amount of

TRIZOL Reagent added is based on the area of the culture dish (1 ml per 10 cm2) and not

on the number of cells present. An insufficient amount of TRIZOL Reagent may result in

contamination of the isolated RNA with DNA.

c.

Cells Grown in Suspension

Pellet cells by centrifugation. Lyse cells in TRIZOL Reagent by repetitive pipetting. Use

1 ml of the reagent per 5-10 × 106 of animal, plant or yeast cells, or per 1 × 107 bacterial

cells. Washing cells before addition of TRIZOL Reagent should be avoided as this

increases the possibility of mRNA degradation. Disruption of some yeast and bacterial

cells may require the use of a homogenizer.

OPTIONAL: An additional isolation step may be required for samples with high content of

proteins, fat, polysaccharides or extracellular material such as muscles, fat tissue, and tuberous

parts of plants. Following homogenization, remove insoluble material from the homogenate by

centrifugation at 12,000 × g for 10 minutes at 2 to 8°C. The resulting pellet contains

extracellular membranes, polysaccharides, and high molecular weight DNA, while the

supernatant contains RNA. In samples from fat tissue, an excess of fat collects as a top layer

which should be removed. In each case, transfer the cleared homogenate solution to a fresh

tube and proceed with chloroform addition and phase separation as described.

2. PHASE SEPARATION

Incubate the homogenized samples for 5 minutes at 15 to 30°C to permit the complete

dissociation of nucleoprotein complexes. Add 0.2 ml of chloroform per 1 ml of TRIZOL

Reagent. Cap sample tubes securely. Shake tubes vigorously by hand for 15 seconds and

incubate them at 15 to 30°C for 2 to 3 minutes. Centrifuge the samples at no more than 12,000

× g for 15 minutes at 2 to 8°C. Following centrifugation, the mixture separates into a lower

red, phenol-chloroform phase, an interphase, and a colorless upper aqueous phase. RNA

remains exclusively in the aqueous phase. The volume of the aqueous phase is about 60% of

the volume of TRIZOL Reagent used for homogenization.

3. RNA PRECIPITATION

Transfer the aqueous phase to a fresh tube, and save the organic phase if isolation of DNA or

protein is desired. Precipitate the RNA from the aqueous phase by mixing with isopropyl

alcohol. Use 0.5 ml of isopropyl alcohol per 1 ml of TRIZOL Reagent used for the initial

homogenization. Incubate samples at 15 to 30°C for 10 minutes and centrifuge at no more than

12,000 × g for 10 minutes at 2 to 8°C. The RNA precipitate, often invisible before

centrifugation, forms a gel-like pellet on the side and bottom of the tube.

4.

RNA WASH

Remove the supernatant. Wash the RNA pellet once with 75% ethanol, adding at least 1 ml of

75% ethanol per 1 ml of TRIZOL Reagent used for the initial homogenization. Mix the sample

by vortexing and centrifuge at no more than 7,500 × g for 5 minutes at 2 to 8°C.

5.

REDISSOLVING THE RNA

At the end of the procedure, briefly dry the RNA pellet (air-dry or vacuum-dry for 5-10

minutes). Do not dry the RNA by centrifugation under vacuum. It is important not to let the

RNA pellet dry completely as this will greatly decrease its solubility. Partially dissolved RNA

samples have an A260/280 ratio < 1.6. Dissolve RNA in RNase-free water or 0.5% SDS solution

by passing the solution a few times through a pipette tip, and incubating for 10 minutes at 55 to

60°C. (Avoid SDS when RNA will be used in subsequent enzymatic reactions.) RNA can also

be redissolved in 100% formamide (deionized) and stored at -70°C (5).

RNA Isolation Notes:

1.

Isolation of RNA from small quantities of tissue (1 to 10 mg) or Cell (102 to 104) Samples:

Add 800 µl of TRIZOL to the tissue or cells. Following sample lysis, add chloroform and

proceed with the phase separation as described in step 2. Prior to precipitating the RNA with

isopropyl alcohol, add 5-10 µg RNase-free glycogen (Cat. No 10814) as carrier to the

aqueous phase. To reduce viscosity, shear the genomic DNA with 2 passes through a 26

gauge needle prior to chloroform addition. The glycogen remains in the aqueous phase and

is co-precipitated with the RNA. It does not inhibit first-strand synthesis at concentrations up

to 4 mg/ml and does not inhibit PCR.

2.

After homogenization and before addition of chloroform, samples can be stored at -60 to -70°C

for at least one month. The RNA precipitate (step 4, RNA WASH) can be stored in 75%

ethanol at 2 to 8°C for at least one week, or at least one year at –5 to -20°C.

3. Table-top centrifuges that can attain a maximum of 2,600 × g are suitable for use in these

protocols if the centrifugation time is increased to 30-60 minutes in steps 2 and 3.

INSTRUCTIONS FOR DNA ISOLATION:

Unless otherwise stated, the procedure is carried out at 15 to 30°C, and reagents are at 15 to 30°C.

Reagents required, but not supplied:

Chloroform

Isopropyl alcohol

75% Ethanol (in DEPC-treated water)

RNase-free water or 0.5% SDS solution [To prepare RNase-free water, draw water into

RNase-free glass bottles. Add diethylpyrocarbonate (DEPC) to 0.01% (v/v). Let stand

overnight and autoclave. The SDS solution must be prepared using DEPC-treated, autoclaved

water.]

After complete removal of the aqueous phase, as described in the RNA isolation protocol, the DNA

in the interphase and phenol phase from the initial homogenate may be isolated. Following

precipitation and a series of washes, the DNA is solubilized in 8 mM NaOH. Full recovery of DNA

from tissues and culture cells permits the use of TRIZOL Reagent for the determination of the DNA

content in analyzed samples (2). Simultaneous extraction of genomic DNA allows for normalization

of the results of Northern analysis per genomic DNA instead of the more variable total RNA or

tissue weight. (Depending on the source, the DNA pellet obtained may require additional

purification (e.g., phenol extraction) prior to other applications.

Reagents required, but not supplied:

Ethanol

0.1 M Sodium citrate in 10% ethanol

75% Ethanol

8 mM NaOH

Unless otherwise stated, the procedure is carried out at 15 to 30°C.

1. DNA PRECIPITATION

Remove the remaining aqueous phase overlying the interphase, and precipitate the DNA from

the interphase and organic phase with ethanol. Add 0.3 ml of 100% ethanol per 1 ml of

TRIZOL Reagent used for the initial homogenization, and mix samples by inversion. Next,

store the samples at 15 to 30°C for 2-3 minutes and sediment DNA by centrifugation at no

more than 2,000

Careful removal of the aqueous phase is critical for the quality of the isolated

× g for 5 minutes at 2 to 8°C.

DNA.

2. DNA WASH

Remove the phenol-ethanol supernatant, and if desired, save it for protein isolation. Wash the

DNA pellet twice in a solution containing 0.1 M sodium citrate in 10% ethanol. Use 1 ml of

the solution per 1 ml of TRIZOL Reagent used for the initial homogenization. At each wash,

store the DNA pellet in the washing solution for 30 minutes at 15 to 30°C (with periodic

mixing) and centrifuge at 2,000 × g for 5 minutes at 2 to 8°C. Following these two washes,

suspend the DNA pellet in 75% ethanol (1.5-2 ml of 75% ethanol per 1 ml TRIZOL Reagent),

store for 10-20 minutes at 15 to 30°C (with periodic mixing) and centrifuge at 2,000 × g for 5

minutes at 2 to 8°C.

An additional wash in 0.1 M sodium citrate-10% ethanol solution is required for large pellets

containing > 200

µg DNA or large amounts of a non-DNA material.

3. REDISSOLVING THE DNA

Air dry the DNA 5 to 15 minutes in an open tube. (DO NOT DRY UNDER

CENTRIFUGATION; it will be more difficult to dissolve.) Dissolve DNA in 8 mM NaOH

such that the concentration of DNA is 0.2 – 0.3 µg/µl. Typically add 300 – 600 µl of 8 mM

NaOH to DNA isolated from 107 cells or 50 – 70 mg of tissue. Resuspending in weak base is

HIGHLY recommended since isolated DNA does not resuspend well in water or in Tris

buffers. The pH of the 8 mM NaOH is only ~9 and should be easily adjusted with TE or

HEPES once the DNA is in solution. At this stage, the DNA preparations (especially from

tissues) may contain insoluble gel-like material (fragments of membranes, etc.) Remove the

insoluble material by centrifugation at >12,000 × g for 10 minutes. Transfer the supernatant

containing the DNA to a new tube. DNA solubilized in 8 mM NaOH can be stored overnight

at 4°C; for prolonged storage, samples should be adjusted with HEPES to pH 7-8 (see table)

and supplemented with 1 mM EDTA. Once the pH is adjusted, DNA can be stored at 4°C or –20°C.

Quantitation and Expected Yields of DNA

Take an aliquot of the DNA preparation solubilized in 8 mM NaOH, mix it with water and measure

the A260 of the resulting solution. Calculate the DNA content using the A260 value for double-stranded DNA. One A260 unit equals 50

µg of double-stranded DNA/ml. For calculation of cell

number in analyzed samples, assume that the amount of DNA per 1 × 106 diploid cells of human, rat,

and mouse origin equals: 7.1

µg, 6.5

µg, and 5.8

µg, respectively (3).

Applications:

Amplification of DNA by PCR:

After redissolving the DNA in 8 mM NaOH, adjust the pH to 8.4 with 0.1 M HEPES (see table).

Add 0.1 to 1.0

µg of the DNA sample to your PCR reaction mixture and perform the standard PCR

protocol.

Restriction endonuclease reactions:

Adjust the pH of the DNA solution to a required value using HEPES (see table). Alternatively,

samples may be dialyzed against 1 mM EDTA, pH 7 to pH 8.0. Use 3-5 units of enzyme per

microgram of DNA. Use the conditions recommended by the manufacturer for the particular

enzyme, and allow the reaction to proceed for 3 to 24 h. In a typical assay, 80-90% of the DNA is

digestible.

pH Adjustment of DNA Samples Dissolved in 8 mM NaOH:

(For 1 ml of 8 mM NaOH use the following amounts of 0.1 M or 1 M HEPES, free acid.)

Final pH 0.1 M HEPES (µl) Final pH 1 M HEPES (µl)

8.4 86 7.2 23

8.2 93 7.0 32

8.0 101

7.8 117

7.5 159

DNA Isolation Notes:

1. The phenol phase and interphase can be stored at 2 to 8°C overnight.

2. Samples suspended in 75% ethanol can be stored at 2 to 8°C for months.

3. Samples dissolved in 8 mM NaOH can be stored overnight at 2 to 8°C. For long-term storage,

adjust the pH to 7-8, and adjust the EDTA concentration to 1 mM.

INSTRUCTIONS FOR PROTEIN ISOLATION:

Proteins are isolated from the phenol-ethanol supernatant obtained after precipitation of DNA with

ethanol (step 1, DNA PRECIPITATION). The resulting preparation can be analyzed for the

presence of specific proteins by Western blotting (2).

Reagents required, but not supplied:

Isopropyl alcohol

0.3 M Guanidine hydrochloride in 95% ethanol

Ethanol

1% SDS

1. PROTEIN PRECIPITATION

Precipitate proteins from the phenol-ethanol supernatant (approximate volume 0.8 ml per 1 ml

of TRIZOL Reagent) with isopropyl alcohol. Add 1.5 ml of isopropanol per 1 ml of TRIZOL

Reagent used for the initial homogenization. Store samples for 10 minutes at 15 to 30°C, and

sediment the protein precipitate at 12,000 × g for 10 minutes at 2 to 8°C.

2. PROTEIN WASH

Remove the supernatant and wash the protein pellet 3 times in a solution containing 0.3 M

guanidine hydrochloride in 95% ethanol. Add 2 ml of wash solution per1 ml of TRIZOL

Reagent used for the initial homogenization. During each wash cycle, store the protein pellet

in the wash solution for 20 minutes at 15 to 30°C and centrifuge at 7,500 × g for 5 minutes at 2

to 8°C. After the final wash, vortex the protein pellet in 2 ml of ethanol. Store the protein

pellet in ethanol for 20 minutes at 15 to 30°C and centrifuge at 7,500 × g for 5 minutes at 2 to

8°C.

3. REDISSOLVING THE PROTEIN PELLET

Vacuum dry the protein pellet for 5-10 minutes. Dissolve it in 1% SDS by pipetting. Complete

dissolution of the protein pellet may require incubating the sample at 50°C. Sediment any

insoluble material by centrifugation at 10,000 × g for 10 minutes at 2 to 8°C, and transfer the

supernatant to a fresh tube. The sample is ready for use in Western blotting or may be stored at

-5 to -20°C for future use.

Protein Isolation Notes:

1. The protein pellet suspended in 0.3 M guanidine hydrochloride-95% ethanol or in ethanol can

be stored for at least one month at 2 to 8°C, or for at least one year at -5 to -20°C.

2. The following protocol is an alternative approach that allows for more efficient recovery of

proteins. Dialyze the phenol-ethanol supernatant against three changes of 0.1% SDS at 2 to

8°C. Centrifuge the dialyzed material at 10,000 × g for 10 minutes. Use the clear supernatant

for Western blotting.

3.

Proteins may be quantified by the Bradford method as long as the concentration of SDS is low

enough (<0.1%) so that it will not interfere. Methods that do not have detergent-interface

problems, and that do not rely on A

cause overestimation of protein concentrations).

260/A280 measurements may be used (traces of phenol may

Troubleshooting Guide:

RNA ISOLATION

•Expected yields of RNA per mg of tissue or 1

× 106 cultured cells

Kidney,

Liver and spleen, 6-10

µ

g

g

µ Placenta,

Skeletal muscles and brain, 1-1.5

3-4

µ Epithelial cells (1

1-4 g

g

µ× 106 cultured cells), 8-15

µ Fibroblasts, (1 × 106 cultured cells) 5-7

g

µ•Low yield

g

Incomplete homogenization or lysis of samples.

•AFinal RNA pellet incompletely redissolved.

260/ARNA sample was diluted in water instead of TE prior to spectrophotometric analysis. Low

280 ratio <1.65

ionic strength and low pH solutions increase absorbance at 280 nm (6,7).

Sample homogenized in too small a reagent volume.

Following homogenization, samples were not stored at room temperature for 5 minutes.

The aqueous phase was contaminated with the phenol phase.

•RNA degradation

Incomplete dissolution of the final RNA pellet.

Tissues were not immediately processed or frozen after removal from the animal.

Samples used for isolation, or the isolated RNA preparations were stored at -5 to-20°C, instead

of -60 to -70°C.

Cells were dispersed by trypsin digestion.

Aqueous solutions or tubes were not RNase-free.

•DNA contamination

Formaldehyde used for agarose-gel electrophoresis had a pH below 3.5.

Sample homogenized in too small a reagent volume.

Samples used for the isolation contained organic solvents (e.g., ethanol, DMSO), strong

• Proteoglycan and polysaccharide contamination

buffers, or alkaline solution.

The following modification of the RNA precipitation (step 3) removes these contaminating

compounds from the isolated RNA. Add to the aqueous phase 0.25 ml of isopropanol followed

by 0.25 ml of a high salt precipitation solution (0.8 M sodium citrate and 1.2 M NaCl) per 1 ml

of TRIproceed with the isolation as described in the protocol. The modified precipitation effectively

ZOL Reagent used for the homogenization. Mix the resulting solution, centrifuge and

precipitates RNA while maintaining polysaccharides and proteoglycans in a soluble form. A

combination of the modified precipitation with an additional centrifugation of the initial

homogenate (note 2, RNA isolation protocol) is required to isolate pure RNA from plant

material containing a very high level of polysaccharides.

DNA ISOLATION

•Expected yields of DNA per mg of tissue or 1

Liver and kidney, 3-4

× 106 cultured cells

µg

Skeletal muscles, brain, and placenta 2-3

µ Fibroblasts,

Cultured human, rat, and mouse cells (1

•Low yield

5-7 g

× 10g

6), 5-7

µg

µ

Incomplete homogenization or lysis of samples.

•AFinal DNA pellet incompletely redissolved.

260/280DNA sample was diluted in water instead of TE prior to spectrophotometric analysis.

ratio <1.70

Phenol was not sufficiently removed from the DNA preparation. Wash the DNA pellet an

•DNA degradation

additional time with 0.1 M sodium citrate in 10% ethanol.

Tissues were not immediately processed or frozen after removal from the animal.

Samples used for isolation, or the isolated RNA preparations were stored at -5 to-20°C, instead

of -60 to -70°C.

•RNA contamination

Samples were homogenized with a Polytron or other high speed homogenizer.

Incomplete removal of aqueous phase.

•Other applications

DNA pellet insufficiently washed with 0.1 M sodium citrate in 10% ethanol.

Prior to use in PCR amplification, adjust the pH to 8.4.

For digestion of the DNA with restriction endonucleases, adjust the pH to the desired value,

use 3-5 units of enzyme per

optimal conditions for the particular enzyme. Typically 80-90% of the DNA is digested.

µg of DNA, and allow the reaction to go for 3-24 hours under

PROTEIN ISOLATION

•Low yield

Incomplete homogenization or lysis of samples.

•Protein degradation

Final DNA pellet incompletely redissolved.

•Band deformation in PAGE

Tissues were not immediately processed or frozen after removing from the animal.

Protein pellet insufficiently washed.

References:

1.

2.

Chomczynski, P., and Sacchi, N. (1987) Anal. Biochem.

3. Ausubel,

Chomczynski, P. (1993)

162, 156.

F.M., , eds. (1990)

Biotechniques 15,Current Protocols in Molecular Biology 532.

4.

Publishing Assoc. and Wiley-Interscience, New York, p.A.1.5.

, Vol.2, Greene

5.

Simms, D., Cizdziel, P.E., Chomczynski, P. (1993) FOCUS® 15, 99.

6.

Bracete, A.M., Fox, D.K., and Simms, D. (1998) FOCUS 20, 82).

7.

Wilfinger, W., Mackey, K. and Chomczynski, P. (1997)

Fox, D.K. (1998) F 37.

BioTechniques 22, 474.

OCUS 20,Teflon® is a registered trademark of E. I. Du Pont de Nemours & Co.

TISSUMIZER®

is a registered trademark of Tekmar Co.

TRIZOL ® is a registered trademark of Molecular Research Center, Inc.

*PCR is covered by a patent held by Hoffman LaRoche Corporation.

Cat No. 15596-026