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The Growth of GM foods

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Title: Slide 1 Author: Caitlin Forsyth Last modified by: Lab Default Created Date: 2/25/2006 2:12:11 AM Document presentation format: On-screen Show – PowerPoint PPT presentation

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Title: The Growth of GM foods

1
The Growth of GM foods

From 1996 to 2003
Global farmland used to grow transgenic crops
increased 40 fold

2
The Genetically Modified Food Debate

Concerned Consumers
New toxins and allergens
Glyphosate
Super Weeds
Loss of bio-diversity in crops
The disturbance of ecological balance
Supporters
Increased yields
Increased nutritional value
Hardy crops
Vaccines
Rapid maturity
More people, fewer resources

3
GM Maize Products

45 of all maize grown in US is GM
cry1A(b) gene
Pesticide
Syngenta, Monsanto, Pioneer Hi-Bred
Midwestern United States
Bar gene
Herbicide resistance
Bayer, Aventis

4
The Development of a Unique Protocol for Use in
Testing for Genetically Modified Ingredients in
Maize Products
Caitlin Forsyth W.F. West High School
5
Purpose

The purpose of this research was to find a
correlation between specific genetic modification
and geographic origin of maize products, using a
specially designed protocol

6
Hypothesis

It was hypothesized that maize products from the
Midwest would be genetically modified, and more
specifically, with the Cry1A(b) gene

7
Methods Procedures

Homogenization of test and control foods
Extraction of DNA
PCR on Extracted DNA
Gel Electrophoresis

8
Experimental Design

Multiple Controls
Positive
Negative
Zein
Selection of test foods
Midwest
West Coast

9
Homogenization of Maize Products

Coffee Grinder
Mini pestle and mortar

10
Extraction of DNA

Bio-Rads InstaGene Matrix
Machery-Nagels Nucleo-Spin Food Extraction Kit
Qiagens Plant Extraction Kit

11
Polymerase Chain Reaction

Test and Control Foods
Zein
CaMV/NOS
Cry1A(b)
Bar
Primer sequences
Oligo analyzer

12
Gel Electrophoresis

The PCR products were run on 2 agarose gels with
a 14-tooth comb
Zein
277 b.p.
CaMV/NOS
203 b.p. CaMV
225 b.p. NOS
Bar
600 b.p.
Cry1A(b)
240 b.p.

13
The First Trial

European Joint Research Council GM Testing
Protocol
Annealing temperatures
Primer sequences
No amplification of Cry1A(b), bar, or zein
Harder than anticipated

14
The Second Trial

Annealing Temperatures
Primer melting temperatures
No amplification of zein, bar, or Cry1A(b)

15
The Third Trial

PCR Optimization
MgCl2
Qiagens Q-Solution
BSA
Amplification of zein, bar, and Cry1A(b) positive
controls
Unable to duplicate results

16
Results-Trial 7
Great Value Corn
Tostitos
CA WA corn
Green Giant
GV Taco Shells
Libby Organic Corn
Organic Tostitos
Safeway Taco Shells
Padrinos
17
Gel Arrangement
1 2 3 4 5 6 7 8 9 10 11
12 13 14
Negative Positive Test food
250 200 150 100 50
CaMV/NOS
Cry1A(b)
Zein
Cry1A(b)
Zein
Bar
18
Tostitos Tortilla Chips

Amplification of zein
Amplication of CaMV/NOS
Non-Specific Amplification Cry1A(b) and Bar

250 200 150 100 50
19
Great Value Taco Shells

No amplification of zein
Amplification of CaMV/NOS
Non-specific amplification of Cry1A(b) and Bar

250 200 150 100 50
20
Subsequent Trials

Second Round PCR
Extraction Techniques
HotStarTaq Polymerase

21
Results-Trial 13
CA WA Corn
Del Monte
Green Giant
Great Value Corn
Safeway Taco Shells
Great Value Taco Shells
Libby Organic Corn
Organic Tostitos
Padrinos
Tostitos
22
Gel Arrangement

Lane 1
50 b.p. ladder
Lane 14
Lambda/HindIII marker
Negative/Positive Controls

23
Tostitos Tortilla Chips

Amplification of 200 base pair band
Same streaking pattern as Cry1A(b) positive
control

250 200 150 100 50
24
Green Giant Canned Corn

No amplification of 200 base pair band
No amplification of zein
Non-specific amplification of Cry1A(b)

250 200 150 100 50
25
Overall Results

CaMV/NOS positive
Great Value Taco Shells
Libby Organic Corn
Padrinos Restaurant Style Tortilla Chips
Tostitos Tortilla Chips
Nonspecific Amplification
Cry1A(b)
Bar

26
Correlation

Geographic Origin
PadrinosCalifornia Texas
Great Value Taco Shells Arkansas
Tostitos Tortilla Chips Texas
Libby Organic Corn New York
Inconclusive correlation

27
Conclusion

Purpose changed
GM testing manual
Became necessary to develop and test new
protocols
Protocol still not completed

28
Limitations

PCR inhibitors
Starch
Highly processed food
Positive Controls

29
Future Research

Touchdown PCR
Third Round PCR
High annealing temperature
Positive control designed primers
Different Taq varieties
DNA repair enzyme
More food samples
Correlation

30
Acknowledgements

Henri Weeks
Dr. Bryony Wiseman
My parents, Norm Carolee Forsyth

31
Questions?
32
Qiagens HotStarTaq Polymerase

Qiagens HotStarTaq Polymerase was used because
it minimizes nonspecific amplification products,
primer-dimers, and background.
MasterMix and PCR reactions can be set up at room
temperature.

33
Qiagens Q-Solution

Modifies melting behavior of DNA
Increases specificity, amplification success

34
MgCl2

Increasing concentration of MgCl2 increases
specificity
Too high of MgCl2 concentration inhibits the
polymerase chain reaction

35
The Bar Gene

Transgenic cells and plants expressing this gene
are resistant to the herbicides Basta (Europe),
Bialaphos (Japan) and Ignite (USA)
Glufosinate ammonium tolerance
Glufosinate chemically resembles the amino acid
glutamate and acts to inhibit an enzyme, called
glutamine synthetase, which is involved in the
synthesis of glutamine
Glufosinate acts enough like glutamate, that it
blocks the enzyme's usual activity

36
Components of a PCR Reaction

The Template DNA
Primers
A Master Mix containing
dNTPs
Buffer
Taq Polymerase

37
What genes are used in GMFs?

Foreign genes are translated into foreign
proteins
Desired effects
Pesticides
BT
More desirable size color, desirable to
consumer
Resistant to harsh environmental conditions
More nutritional value, altered vitamin, mineral,
and fat contents
Food to vaccinate against diseases
Banana that produces an antigen found in the
outer coat of the Hepatitis B virus

38
DNA Extraction

Physically break cell wall
Lysis buffer
Opens cell
DNA binds to membrane
Wash with solutions containing ethanol to wash
away impurities
Elution

39
BSA

Reduces the frequency of primer dimers
Reduces PCR inhibition

40
Glyphosate

On the market now, Monsanto
Glyphosate kills tadpoles, decline in frog
population
Hardell and Eriksson
link between glyphosate and lymphoma, link was
not statistically significant and was within the
realm of random variation.

41
Taq Polymerase

Isolated from bacterium that lives in heat vents
and hot springs
Commerically sold Taq DNA polymerase (low
fidelity) has an error rate of one in 8 million
nucleotides
Adds nucleotides to the primer ends
Proofreading mechanism
Vent
Pfu

42
How Does PCR Work?
Chromosome
Problem How do we detect the presence of a
modified sequence within an organisms genome?
Plant Cell
Cauliflower Mosaic Virus Promoter Sequence 203
b.p.
43
Polymerase Chain Reaction
44
Cauliflower Mosaic Virus Promoter Sequence 203
b.p.
After 30 cycles
Millions of copies of the 203 b.p. virus promoter
sequence common in many GMOs
45
Zein Gene

Naturally occurring maize gene
Class of protein
Used to coat paper cups, buttons, adhesives
Can replace gum base in chewing gum

46
Cry1A(b) gene

The cry1Ab gene produces protein Cry1Ab
Cry proteins, of which Cry1Ab is only one, binds
to the lining of the gut of lepidopteran insects
Pores are formed that disrupt ion flow, causing
gut paralysis and cell lysis and eventual death

47
GM testing of milk/animal products

GM Protein-based testing
GM hormone testing

48
Gel Electrophoresis

DNA (sugar-phosphate backbone) negatively charged
Loaded on negative side, attracted to positive
side
Gel forms porous matrix
Electric current carried through running buffer
Small fragments go through faster, end of gel
Ethidium bromide stain

49
Organic Foods

Modified genes were found in normal plants more
than 13 miles away from the source
Products labeled "organic" must consist of at
least 95 percent organically produced ingredients

50
Nonspecific PCR Product

PCR cycling conditions not optimal
Annealing temperature too low
Primer concentration not optimal
Primers degraded
Primer design not optimal
More bases in primer design

51
Why are some genes easier to amplify than others?

Primer design optimal
No self-diming or hetero-diming
Primer concentration
Annealing temperature
PCR cycling conditions
CaMV/NOS primers took 6 months to optimize
Some regions of DNA have a secondary structure
that affects the binding and annealing of the
primers

52
Primer Length

1 in 4(number of bases) probability that the
primers will match to another place
For example the difference between 20 and 24
bases
420
1.1x1012
424
2.81x1014
Difference
2.80x1014

53
Smeared PCR Product

Too much starting template
Carryover contamination
Enzyme concentration too high
Too many cycles

54
Little or no PCR Product

Pipetting error, missing reagent
PCR cycling conditions not optimal
Primers degraded
Problems with starting template
Enzyme concentration too low
Insufficient number of cycles
Extension time too short
Primer design not optimal

55
Dangers of GM Food

Health effects
Puztai
Rats, GE potatoes with lectin, intestinal
problems
Cornell U.
Moths, milkweed with Bt pollen, death and lack of
maturity
Increased use of chemicals on crops

56
Labeling GMOs Worldwide

Europe
Foods containing over 1 labeled as GMO
Food crises in 1990s
Asia
Similar to Europe
No threshold established
Thailand non-GMO zones
United States
Foods with less than 5 GMOs may be labeled as
GMO-free, 3 counties in CA have banned production
of GM crops
World Trade Organization
Banning GM crops
Unnecessary obstacle to international trade

57
Methods of Genetically Engineering Food