David A. Palmer, Ph.D.

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Title: David A. Palmer, Ph.D.

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Real-Time PCR

David A. Palmer, Ph.D.
Technical Support, Bio-Rad Laboratories
Adjunct Professor, Contra Costa College

3
Objectives

Today well talk about Real-Time PCR
What is real-time PCR used for?
How does real-time PCR work?
What chemicals and instruments are used to detect
DNA?
What does real-time data look like?
How can we demonstrate real-time PCR in the
classroom?

4
Part 1 What is Real-Time PCR and what is it
used for?
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What is Real-Time PCR?

PCR, or the Polymerase Chain Reaction, is a
process for the amplification of specific
fragments of DNA.
Real-Time PCR a specialized technique that allows
a PCR reaction to be visualized in real time as
the reaction progresses.
As we will see, Real-Time PCR allows us to
measure minute amounts of DNA sequences in a
sample!

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What is Real-Time PCR?

Conventional PCR
tells us what.
Real-Time PCR
tells us how much.

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What is Real-Time PCR used for?

Real-Time PCR has become a cornerstone of
molecular biology. Just some of the uses
include
Gene expression analysis
Cancer and Drug research
Disease diagnosis and management
Viral quantification
Food testing
Percent GMO food
Animal and plant breeding
Gene copy number
Forensics
Sample identification and quantification

8
Real-Time PCR in Gene Expression Analysis

Example BRCA1 Expression Profiling
BRCA1 is a gene involved in tumor suppression.
BRCA1 controls the expression of other genes.
In order to monitor level of expression of BRCA1,
real-time PCR is used.

Determine gene expression and publish scientific
paper!
Real-Time PCR
DNA
BRCA1
mRNA
Protein
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Real-Time PCR in Disease Management

Example HIV Treatment
Drug treatment for HIV infection often depends on
monitoring the viral load.
Real-Time PCR allows for direct measurement of
the amount of the virus RNA in the patient.

Real-Time PCR
Viral RNA
Measure amount of virus, adjust prescriptions.
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Real-Time PCR in Food Testing

Example Determining percentage of GMO food
content
Determination of percent GMO food content
important for import / export regulations.
Labs use Real-Time PCR to measure amount of
transgenic versus wild-type DNA.

Real-Time PCR
wt DNA
GMO DNA
International shipments depend on results!
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Real-Time PCR in Forensics

Example Real-Time PCR in Forensic Analysis!
Stain Identification
New Real-Time methods can be directly used to
identify the composition of unknown stains, with
much better accuracy than traditional
color-change tests.
DNA Quantification
Since standard forensic STR Genotyping requires
defined amounts of DNA, Real-Time PCR can be used
to accurately quantify the amount of DNA in an
unknown sample!

What is it ??
Enough DNA to ID ??
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Part 2 How does Real-Time PCR work?
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How does real-time PCR work?

To best understand what real-time PCR is, lets
review how regular PCR works...

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The Polymerase Chain ReactionHow does PCR work??
d.NTPs
Primers
Thermal Stable DNA Polymerase
Add to Reaction Tube
Denaturation
Annealing
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The Polymerase Chain ReactionHow does PCR work??
Extension
Extension Continued
Repeat
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The Polymerase Chain ReactionHow does PCR work??
Cycle 2 4 Copies
Cycle 3 8 Copies
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How does Real-Time PCR work?

So thats how traditional PCR is usually
presented.
In order to understand real-time PCR, lets use a
thought experiment, and save all of the
calculations and formulas until later

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Imagining Real-Time PCR

To understand real-time PCR, lets imagine
ourselves in a PCR reaction tube at cycle number
25

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Imagining Real-Time PCR

Whats in our tube, at cycle number 25?
A soup of nucleotides, primers, template,
amplicons (the amplified DNA product), enzyme,
etc.
1,000,000 copies of the amplicon right now.

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Imagining Real-Time PCRHow did we get here?

What was it like last cycle, 24?
Almost exactly the same, except there were only
500,000 copies of the amplicon.
And the cycle before that, 23?
Almost the same, but only 250,000 copies of the
amplicon.
And what about cycle 22?
Not a whole lot different. 125,000 copies of the
amplicon.

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Imagining Real-Time PCRHow did we get here?

If we were to graph the amount of DNA in our
tube, from the start until right now, at cycle
25, the graph would look like this

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Imagining Real-Time PCRHow did we get here?
?

So, right now were at cycle 25 in a soup with
1,000,000 copies of the target.
Whats it going to be like after the next cycle,
in cycle 26?

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Imagining Real-Time PCRSo where are we going?

Whats it going to be like after the next cycle,
in cycle 26?
Probably there will be 2,000,000 amplicons.
And cycle 27?
Maybe 4,000,000 amplicons.

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Imagining Real-Time PCRSo where are we going?

Whats it going to be like after the next cycle,
in cycle 26?
Probably there will be 2,000,000 amplicons.
And cycle 27?
Maybe 4,000,000 amplicons.
And at cycle 200?
In theory, there would be 1,000,000,000,000,000,00
0,000,000,000,000,000,000,000,000,000,000,000,000,
000 amplicons
Or 1035 tons of DNA
To put this in perspective, that would be
equivalent to the weight of ten billion planets
the size of Earth!!!!

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Imagining Real-Time PCRSo where are we going?

A clump of DNA the size of ten billion planets
wont quite fit in our PCR tube anymore!!!
Realistically, at the chain reaction progresses,
it gets exponentially harder to find primers, and
nucleotides. And the polymerase is wearing out.
So exponential growth does not go on forever!

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Imagining Real-Time PCRSo where are we going?

If we plot the amount of DNA in our tube going
forward from cycle 25, we see that it actually
looks like this

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Imagining Real-Time PCRMeasuringQuantities

How can all this be used to measure DNA
quantities??

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Imagining Real-Time PCRMeasuringQuantities

Lets imagine that you start with four times as
much DNA as I do.
Picture our two tubes at cycle 25 and work
backwards a few cycles.

Cycle 25
Cycle Me You
25 1,000,000 4,000,000
24 500,000 2,000,000
23 250,000 1,000,000
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Imagining Real-Time PCRMeasuringQuantities

So, if YOU started with FOUR times as much DNA
template as I did
Then youd reach 1,000,000 copies exactly TWO
cycles earlier than I would!

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Imagining Real-Time PCRMeasuringQuantities

What if YOU started with EIGHT times LESS DNA
template than I did?

Cycle 25
Cycle Me You
25 1,000,000 125,000
26 2,000,000 250,000
27 4,000,000 500,000
28 8,000,000 1,000,000
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Imagining Real-Time PCRMeasuringQuantities

What if YOU started with EIGHT times LESS DNA
template than I did?
Youd only have 125,000 copies right now at cycle
25
And youd reach 1,000,000 copies exactly THREE
cycles later than I would!

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Imagining Real-Time PCRMeasuringQuantities

We can easily see that the left-right shift in
the curves is related to the starting quantity of
DNA!
Cq (Cycle Quantity) values identify the curve
positions, based on where they cross a threshold.
DNA Quantity and Cq value are related as
Quantity 2Cq

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23
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Imagining Real-Time PCRMeasuringQuantities

We can plot the Cq value versus the Log Quantity
on a graph

and calculate the quantity of any unknown
right off of the line!!

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Real-Time PCRSensitivity

How sensitive is Real-Time PCR?
Ultimately, even a single copy can be measured!
In reality, typically about 100 copies is around
the minimum amount.
One hundred copies of a 200-bp gene is
twenty attograms (2 x 10-17 g) of DNA!
this is just 2/100ths of a microliter of blood!

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Part 3 How do we detect and measure DNA?
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How do We Measure DNA in a PCR Reaction?

We use reagents that fluoresce in the presence of
amplified DNA!

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Measuring DNA Ethidium Bromide

Ethidium Bromide
common and well known
- toxic, not very bright

http//www.web.virginia.edu/Heidi/chapter12/chp12.
htm
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Measuring DNA SYBR Green I

SYBR Green I
Bright fluorescence!
Low toxicity!

Ames test results from Molecular Probes Singer et
al., Mutat. Res. 1999, 439 37- 47
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Fluorescent Dyes in PCRIntercalating Dyes
SYBR Green in Action!
PCR makes more double-stranded DNA
SYBR Green dye binds to dsDNA
When illuminated with light at 490nm, the
SYBRDNA complex fluoresces at 520nm.
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Fluorescent Dyes in PCROther Options
Even more ways to detect PCR products

Other Intercalating Dyes
- Eva Green
Probes
- TaqMan Probes
Primer/Probe Combinations
- Scorpions
- LUX Primers

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What Type of Instruments are used with Real-Time
PCR?

What about the Instruments?
Real-time PCR systems consist of THREE main
components
Thermal Cycler (PCR machine), linked to a
Optical Module (to detect fluorescence in the
tubes during the run), linked to a
Computer (to translate the fluorescence data into
meaningful results).

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What Type of Instruments are used with Real-Time
PCR?

A good example is the MiniOpticon real-time
instrument.

Optical Module Thermal Cycler Base
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What Type of Instruments are used with Real-Time
PCR?

One more example is the Bio-Rad CFX-Touch
real-time PCR instrument.

Optical Module Thermal Cycler Base
The CFX module scans the PCR plate with LEDs and
records fluorescence in each well at each PCR
cycle.
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What Type of Software is used with Real-Time PCR?

The computer, running real-time software,
converts the fluorescent signals in each well to
meaningful data.
Workflow
Set up PCR protocol.
Set up plate layout.
Collect data.
Analyze data.

2
3,4
1
45
Part 4 What does actual real-time data look
like, and what are melt curves?
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Real-Time PCRActual Data

This is some actual data from a recent real-time
PCR run.
Data like this can easily be generated by
preparing a dilution series of DNA.

c366939
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Real-Time PCRFinal Product

The final product of real-time PCR is a table of
Ct values, from which amounts of DNA can be
determined.

Well Fluor Content Cycle Quantity ( Cq )
A03 SYBR Std-1 8.90
A04 SYBR Std-2 12.20
A05 SYBR Std-3 15.34
A06 SYBR Std-4 18.77
A07 SYBR Std-5 21.84
A08 SYBR Std-6 25.24
A09 SYBR Std-7 28.82
B03 SYBR Std-1 8.85
B04 SYBR Std-2 12.12
B05 SYBR Std-3 15.31
B06 SYBR Std-4 18.69
B07 SYBR Std-5 21.76
B08 SYBR Std-6 25.24
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Real-Time PCRMelt Curves

The fluorescence data collected during PCR tells
us how much
. but there is another type of analysis we
can do that tells us what!

c366939
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Melt CurvesBasics

Melt curves can tell us what products are in a
reaction.
The principle of melt curves is that as DNA melts
(becomes single stranded), DNA-binding dyes will
no longer bind and fluoresce.

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Melt CurvesBasics

Melt curves can tell us what products are in a
reaction.
PCR products that are shorter or lower GC will
melt at lower temperatures.
Different PCR products will therefore have
different shaped curves.

RFU vs Temp
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Melt CurvesTypical Data

For convenience, we typically view the derivative
(slope) of the actual melt curve data.
The resulting graph looks like a chromatogram,
with peaks that represent different PCR products.

Teaching Tip Use Melt Curves to bring up a good
discussion of why different DNA sequences will
melt at different temperatures! Talk about
base-pairing, secondary structure, energy levels,
etc!
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Melt CurvesHigh-ResolutionAnalysis

The new field of Precision Melt Analysis even
allows differentiation between PCR products based
on a single-base pair mismatch!
PMA/HRM is now used in mutation screening,
detection of biological diversity, and genetic
analysis.

PCR melt data from different organisms is first
collected.
Then normalized.
Then the organisms are compared against each
other.
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Part 5 How can we demonstrate real-time PCR in
the classroom?
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Crime Scene Investigator Kitin Real-Time

CSI MATERIALS REQUIRED
To run the CSI Kit in real-time, only a few
additional items are needed
iQ SYBR Green Supermix
and appropriate tubes/caps
A real-time PCR instrument

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Crime Scene Investigator Kitin Real-Time

CSI INSTRUCTIONS
An Application Note and a Starter Kit are
available (166-2660EDU)
The PCR reactions in the CSI kit can be run in
real-time as an add-on to the regular kit.

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Crime Scene Investigator Kitin Real-Time

CSI FINAL RESULTS
The Crime Scene Real-Time Extension is great for
first-time users!!
Teach PCR, Real-Time, Melt Curves, etc!

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GMO Investigator Kitin Real-Time

GMO MATERIALS REQUIRED
To run the GMO Kit in real-time, only two
additional items are needed
iQ SYBR Green Supermix
and appropriate tubes/caps
A real-time PCR instrument

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GMO Investigator Kitin Real-Time

GMO INSTRUCTIONS
An Application Note and Starter Kit (166-2560EDU)
are available
Basically, run GMO kit with real-time reagents on
a real-time instrument.

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GMO Investigator Kitin Real-Time

GMO FINAL PRODUCT
Ultimately, you can even calculate the percentage
GMO content in actual food samples!
The GMO Real-Time extension is perfect for more
advanced users!

Food Plant Cq GMO Cq Delta Cq Plant Delta Cq GMO GMO Plant ddCq Ratio 2ddCt Ratio
100 GMO 23 27 0 0 0 1 100
Non-GMO 24 39 -1 -12 -11 0.0004 0.04
Product A 22 30 1 -3 -4 .0625 6.3
Product B 25 29 -2 -2 0 1 100
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Real-Time in the ClassroomGetting Started

Getting started with teaching Real-Time PCR in
the classroom is easy !
Use the Crime Scene Real-Time starter kit.
Use the GMO Investigator Real-Time kit.
Use your own PCR primers and templates with SYBR
Green Supermix.
Its nothing more complicated than using a
slightly different polymerase supermix, correct
plastics, and running on a real-time instrument !

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Why Real-Time in the Classroom is Cool!

Real-Time PCR in the classroom is cool for a
number of reasons!
Instant Results! You can see amplification
within minutes of starting the PCR run. No
waiting until next lab period and waiting for
gels to run.
What-Will-Happen-Next Factor! Because samples
amplify at different times, many students will
want to wait for their sample to amplify so
they can see what happens!
Demystifying the Black Box! Now students can see
what happens inside the PCR machine!
Finally a way to connect Computers and Biology!
Many computery students get really excited to
see the computer control of the instrument and
data collection / analysis!

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Conclusions

Weve covered the following topics today
What is real-time PCR used for?
How does real-time PCR work?
What chemicals and instruments are used to detect
DNA?
What does real-time data look like?
How can we demonstrate real-time PCR in the
classroom?

63
Resources and References

David Palmer
David_Palmer_at_bio-rad.com
Bio-Rad Technical Support
1(800)4BIORAD
consult.bio-rad.com
Bio-Rad Explorer website www.explorer.bio-rad.com
Bio-Rad Explorer email biotechnology_explorer_at_bio
-rad.com
Crime Scene Investigator PCR Basics Kit Real-Time
PCR Application Note
Bulletin 166-2505
GMO Investigator Kit Real-Time PCR Application
Note
Bulletin 166-2605
Real-Time PCR Applications Guide
Bulletin 5279

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Real-Time PCRPractical Exercise!
65

Today well use the DNA in the Crime Scene Kit to
make some dilutions for our real-time experiment!
Each workgroup will have DNA from the Crime Scene
kit that has been diluted 110, 1100, 11000,
110000, or undiluted. This is your Unknown
DNA.
Each workgroup will prepare four real-time PCR
reactions
Unknown DNA (replicate 1)
Unknown DNA (replicate 2)
Unknown DNA diluted 1100 (replicate 1)
Unknown DNA diluted 1100 (replicate 2)
If all goes well, youll be able to tell from the
Cq values
Which unknown DNA you started with,
How accurate your pipetting is,
Whether your mini-dilution series demonstrates
high-efficiency PCR.

Todays Experiment An Overview
66

Step 1 DNA Dilutions
Dilute your Unknown DNA 1100.
Mix 1 ul of your DNA (screw-cap tube labelled
1-5) into 99 ul of water (screw-cap tube labelled
W).
Step 2 Prepare your PCR Tubes
Add 20 ul of the spiked SYBR Green Supermix (from
the screw-cap) tube labelled SMX to four PCR
tubes.
Step 3 Add DNA to your PCR Tubes
Add 20 ul of your DNA samples to each PCR tube
Unknown Replicate A
Unknown Replicate B
Unknown 1100 Replicate A
Unknown 1100 Replicate B
Mix gently, avoiding bubbles!
Label appropriately.
Step 4 Cap and Load the PCR Tubes
Place the optically-clear flat caps on the tubes.
Place your reactions in the real-time PCR
machine.

Todays Experiment Step-By-Step
67

Our PCR protocol will look like this
1. 95C for 3 min (activates Taq)
2. 95C for 10 sec (denatures)
3. 52C for 30 sec (extend / anneal)
4. Plate read (captures fluorescence data)
5. Goto Step 2 for 39 more times

Todays Experiment PCR Protocol
68
Real-Time PCR

David A. Palmer, Ph.D.
Technical Support, Bio-Rad Laboratories
Adjunct Professor, Contra Costa College

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BONUS How do we optimize Real-Time PCR and
troubleshoot problems?
70

Optimization of real-time PCR reactions is
important
Since real-time PCR calculations are based on a
doubling of product every cycle, if the reaction
isnt optimized, this doubling will not occur.

Optimization Why?
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A well-optimized reaction will have evenly spaced
standard curves with tight replicates
At 100 efficiency, 10-fold serial dilutions will
be spaced 3.3 cycles apart from each other.

Optimization Example
72

Optimization is normally done as follows
Design multiple primer sets.
Empirically test each primer set with a standard
curve.
Select best primer set, then run a temperature
gradient experiment to determine best annealing
temperature.
Standard curves are ideal for assessing
optimization.

Optimization Basics
73

Why is it important for teachers to be able to
solve real-time PCR problems?
Help students have better success with their
projects!
Preventing problems at the start can help avoid
lost experiments and reagents!
Being able to explain unusual results leads to
great teaching opportunities!

Trouble-shooting Skills Why?
Teaching Tip Very often a students first
real-time data isnt perfect this makes for a
great chance to teach better pipetting skillls,
experimental design, etc!
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Trouble-Shooting