Transcript Isolating Total RNA? Scott Tighe 802-656-2557 HSRF 305 RNA Structure Major Types mRNA-transcription rRNA5s,5.8s,16s, 18s,23s,26s 28s tRNA-Involved in PS Other ncRNAmiRNA, Different from DNA has 2’OH Group! siRNA snRNA snoRNA SmY scaRNA gRNA RNase P RNase MRP.

Isolating Total RNA?
Scott Tighe
802-656-2557
HSRF 305
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RNA Structure
Major Types
mRNA-transcription
rRNA5s,5.8s,16s, 18s,23s,26s
28s
tRNA-Involved in PS
Other ncRNAmiRNA,
Different from DNA
has 2’OH Group!
siRNA
snRNA
snoRNA
SmY
scaRNA
gRNA
RNase P
RNase MRP
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Degradation of RNA-Two Major Catagories
Catalytic/ Enzymatic
RNases
-Catalytic His 12 and His 119, produce a 2’-3’ cyclic
phosphate intermediate similar to chemical catalysis
Ribozymes-RNase P
Chemical Catalysis by
Acid, Base, Divalent Ion
2’ oxygen attacks the adjacent phosphate
2’ OH transesterification
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Yingfu Li, and Ronald R. Breaker J. Am. Chem. Soc., 1999, 121 (23), 5364-5372
Why Total RNA?

Not all transcripts have poly A tail- ie mitochondrial

RNA assessment is more determinative
 rRNA subunit have decrete peaks when running a gel or Bioanalyzer
Total RNA
mRNA

Recovery of special RNA’s such as miRNA, NC RNA, nuclear RNA ect

mRNA recovery kits also recover rRNA anyway
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General RNA Handling
Reagents and Equipment-Considerations:
All reagents MUST be RNase-free
Use gloves that are periodically treated with RNase Zap
Perform all work in a hood
Biosafety
Laminar flow
PCR hood
DO NOT use a fume hood
Use aerosol resistant pipet tips ONLY
Prepare all surfaces and pipets by treating with RNAse Zap
All utensils [scissors, scalpels, tweezers] should be scrubbed clean,
sprayed with RNase Zap, soaked in ETOH and flame sterilized before
a surgery
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General RNA Handling
Prepare daily aliquots of RNase-free water. I aliquot 10-20
tubes each week and discard half way through the day.
Diethylpyrocarbonate [DEPC]-treated water is NOT an
inhibitor for RNases, but rather DEPC is a chemical added to
water to eliminate RNases. After autoclaving [or when
purchased], no DEPC resides in the water.
When opening and closing tubes, be careful not to bump the
inner rim of your tubes.
Use a RNase Inhibitor if allowable by
downstream reactions
RiboLock
Superase
others
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Why an RNase Inhibitor?
RNase Test
Time-0
No RI
With RI
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RNases are almost everywhere
Results from an RNase test system
Surface treated RNase A
followed by Decontamination
Several RNase Inhibitors
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RNA Extraction Systems
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Silica Column-based
 Most use 4M guanidine isothiocyanate [GCN] chaotropic salt
system that denatures RNases without the use of phenol
 RNA is precipitated with ethanol and bound to silica [Si-O-H],
washed, and eluted with water.
PROS
Easy to perform
Compatible with Shedder column
No precipitation rxn
Very clean RNA
Compatible with FastPrep
DNase on the column
CONS
Lipids will interfere and inhibit
Will not isolate MiRNA
Will not isolate RNA <200bp
Lower yield than Trizol
Salts may be left behind
RLT Poor storage integrity at -80
Abrasives can end up in final sample
heavy DNA contamination problems
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RNA Isolation and Purification Systems-[Columnbased]
RNeasy Micro kit [74004]
Small elution volumes 10-15ul for 10ug
Good for FACS samples, LCM, or limited cell
On-column DNase treatment
RNeasy Mini Kit [74104]
Standard Elution volume of 30-50ul for 100ug
General use column
On column DNase treatment
Lipid or Fiber kits too
RNeasy Midi and Maxi Kit
Large elution volumes 150-800ul for 1mg of RNA
USB Corp Prep-Easy Kit
Invitrogen Pure Link micro
Ambion RNAqueous
Zymo Corp-Not recommended
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Trizol-based Reagents
Phenol-Guanidine reagent
TriZol
TriSure
Tri-Reagent
Purezol
QiaZol
Three types
Trizol – Standard-1:9 ratio must be maintained [10% sample]
Trizol LS -Concentrated-1:3 ratio must be maintained [33% sample]
Trizol BD-designed specifically for blood
Remove extracellular biomolecules with chloroform or bromochrolopropane
Requires a precipitation reaction
Use Axygen MCT175C ultra clear tubes
better pelleting
easier to see
May add Pellet Paint, GlycoBlue to precipitation reaction for low [ ] of RNA
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Hybrid Systems
 Use both a Trizol (guanidine-phenol) reagent and silica
column
 Trizol Plus system [Invitrogen]
 Qiagen RNeasy Lipid Tissue Mini Kit
 Bio-Rad Aurum Total RNA Fatty and Fibrous Tissue Kit
 Home Made:
 Perform the standard Trizol
 Transfer Aqueous phase to new tube
 Add 1.5x volume of 100% ETOH
 Apply to column
 Follow standard column proceudures
 Sometimes leaves a Trizol residue on low recovery samples
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Considerations on which system to use
TriZol Applications
Tissues high in lipid and other cellular biomolecules will require Trizol
because of potential interferences of the Si-OH
Trizol has a higher recovery of RNA then RNeasy columns but not
useful for very small amounts of RNA [+/-]
Must be cleaned and DNase-treated using column
Use of Bromochloropropane instead of chloroform for higher purity.
260/280 ratios are often 1.6-1.8 with chloroform and 1.8-2.0 for BCP.
loss of the 28S subunit for solid tissue
Advantageous when grinding matrix is hard to remove- it spins out
Can recover RNA and DNA
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Considerations on which system to use
Silica Column-based Applications [RNeasy]
General use and rapid
No precipitation reaction need
Optimized columns for very small concentrations
On-column one step DNase Treatment
No Phenols or organic solvents
Grinding matrix can end up in the sample
Recoveries of approximately 60% of Trizol (we’ve seen)
DNase-treatment will generally reduce yield by 30% or so
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Considerations on which system to use
Silica Column-based Applications [RNeasy]…continued
Use either centrifuge or vacuum manifold-Multiple loadings
Heat elution water to 60C will increase yield
Do not spin with column open
260/280 ratios are often above 2.00
If using MinElute or MicroElute columns-be aware of the o-ring-it
catches and retains liquid that can get into your final sample
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Extracting RNA
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Extracting RNA from Tissue
 RNA integrity is a function of tissue type and handling!
 Column or Trizol or ….Trizol follow by a column clean-up
 Know your tissue characteristics before starting
High RNase content tissues
Spleen
Pancrease
Intestine
Thymus
Connective tissues, collagen, protein, glycogen, lipids can
interfere with silica column
Brain
Liver
Heart
Muscle
Adipose
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Extracting RNA from Tissue
Use fresh tissue when possible
Use a hood
Use only utensils that are disposable RNase-free or treated with RNase
Zap,ETOH, and flame sterilized!!!
Take special precautions when working with challenging tissues such as
glazing tissue with RNase inhibitor
Place directly into extraction reagent and extract immediate [i.e. homogenize]
 GCN
 TriZol
DO NOT overload the extraction reagent
Interferance of DNA, lipids or polysaccharide can inhibit silica reaction
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Extracting RNA from Tissue- Types of homogenization
 Traditional mortor and pestle with LN2
 Liquid Nitrogen is not always RNase-free
 Difficult to make sterile and RNase-free
 Poly-tron with new tips or RNase-free blades
 Not optimized for very small quantities
 Sometimes difficult to make RNase-free
 Mini motorized pestle
 With or without abrasive
 All RNase-free disposable
 Impactor [bio-pulverizer]
 French Press
 Biomasher columns
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 FastPrep System - Mini-bead beater




Automated, fast, RNase-free
Uses screw cap 2ml tubes, 15ml and 50ml and
optional abrasive for homogenizing tough tissue
Excellent for bacterial extractions
 In Room HSRF 305-Sign up
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Extracting RNA from adherent cells
Directly from plate or dish
Similar for both Trizol and RNeasy system
Do not trypsinize
Remove growth media and washing with PBS (with or w/o RI)
Add enough extraction reagent fro the number of cells
Vortex plate directly
Follow standard operating procedure
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Extracting RNA from other Sources
Suspended mammalian cells
Centrifuge to a pellet
Wash with PBS(RI) to remove serum and media
Add extraction reagent and vortex
Follow SOP
 Viability is key to recovering intact RNA- Trypan or Eosin
 Bacteria and yeast RNA’s are best recovered during early log phase!
 Heating of Trizol or RLT buffer to 50C
 May require FastPrep with abrasive
 Cell wall digestion (Lyticase, Prok, Lysozyme)
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Quality Control of RNA
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Quality Control of RNA
 Consider running an RNase-free gel
 Look for gDNA
 Look for rRNA bands
 We use the E-gel and FlashGels
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Measure your RNA on the Nanodrop and Bioanalyzer
 Can not distinguish DNA from RNA
 Can not distinguish degraded RNA from “good” RNA
Good RNA
RNA prep
with mostly
gDNA from
Neutrophils
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Good vs Degraded RNA
Thing are not always as they appear- These look great on the nanodrop… but….
are they?
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Expected Yield
 Expected yield is very important!!!
 Just getting “enough” RNA is not always ok
 Actively growing mammalian cells contain 1-10 pg/cell
 Calculate your expected RNA recovery
 If you are way below your expected yield than….
 Selectively recovered RNA from weak or apoptotic
cells
 Selectively recovered RNA from G0 or G2M
 Will significantly impact gene expression data
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Problematic Nanodrop Traces
Sample is NOT 183 ng/ul Actually 38ng/ul as per Qubit Spectrofluoromater
272 nm peak is skewing data
260
272
RNA
TRZ
How will this affect
downstream processes
such as RT-qPCR if
one assumes equal
RNA input to a cDNA
reaction?
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Nanodrop Spectra
EDTA
GUANHCL
RLT
Trizol
GUANISOThio
Tween 20
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Nanodrop Spectra
Glycogen
PCI
Amm. ace
MES
Salt
Sod. ace
Alginate
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Nanodrop Spectra
Residual
Trizol
RNase
Inhibitor
ETOH
Tris
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Round table discussion
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FACS and LCM
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FACS sorted cells and RNA
1] FACS must be RNase-free by bleach and other treatments
2] Bacterial contamination in sheath tanks and dip tubes can cause
RNases
3] Hold back cells –check viability- extract RNA as a pre-sort control
4] Add Superase or RiboLock to sort tube and pre-sort tube
containing cells
5] Use RNase-free tubes to sort
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6] Sort into an exact volume of ice cold extraction reagent
 Trizol LS
 RLT buffer [RNeasy Micro]
 Media or buffer with or without Superase
7] After sorting measure the total volume and add the necessary
volume of reagent to obtain the correct ratio of extraction
reagent to sort liquid
8] Consider acceptable sort volumes
9] Extract immediately-do not store cells in extraction buffer at 80
10] DNase-treatment causes RNA losses using RNeasy
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LCM and RNA

Test tissue section before starting by aseptically removing and extracting a
small section. DO NOT LET FROZEN TISSUE THAW!

FFPE tissues often yield no usable RNA and testing its condition before the
start is a good idea

Know what level of degradation your downstream application can tolerate

Fresh frozen tissues perform well

Use RNase Zap-ETOH treated microtome with new blade during sectioning

Use RNase –free slides, tweezers, materials
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LCM
Scape a small section from the prepared slide and extract as a control
Prepare all staining and dehydration reagents from RNase-free reagents and DEPC
water
Collect one LCM cap from large area of cells as a control-non-specific cells
Collect target cells and transfer cap to tube containing extraction agent-vortex
Extract immediately
We have had good luck with RNeasy micro and Pico Pure kits
Omit DNase step to increase recovery when allowable
Extract several caps into one extract buffer or several extract buffers and combine
to increase yield
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Thank you for your attention!
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