Techniques used to make transgenic cows
Scientists producing transgenic cows use a range of techniques including DNA cloning, restriction enzyme digests, ligation, polymerase chain reaction (PCR), transfection, nuclear transfer and in vitro embryo production.
Scientists at AgResearch have successfully generated transgenic cows that produce extra proteins in their milk using the 7 steps described below.
Step 1. Designing the gene construct
- an antibiotic resistance gene – to select cells that have taken up the gene construct
- a tissue-specific promoter sequence – to signal the start of expression of the protein in cells of the appropriate tissue, for example, in mammary cells in lactating cows
- the desired gene – for example, bovine casein or human myelin basic protein
- a stop sequence – to define the end of the information for making the protein.
Step 2. Sourcing the transgene
In the past, the gene would have been extracted from the source organism’s DNA. Now, however, if the desired gene sequence is known, it can simply be synthesised in a lab. There are companies that make genes to order within a couple of weeks.
Step 3. Making the gene construct
The gene is usually supplied in a vector. A vector is a small piece of DNA, often a plasmid, into which a foreign piece of DNA can be inserted. When the gene of interest is in a vector, it can be sent from one lab to another, it can be stored, it can be manipulated or it can be used to transform bacteria to produce more copies of the gene of interest.
Vectors have multiple restriction enzymes sites (also called multiple cloning sites) so the gene can be inserted into the vector and then cut out from the vector using restriction enzymes.
Get information sheet: Restriction enzymes
After the gene is cut from the vector, it is then pasted into the multiple cloning site of the gene construct using a method known as ligation.
Get information sheet: DNA ligation
Step 4. Transfecting bovine cells
The gene construct is incorporated into the genome of a bovine (cow) cell using a technique called transfection. During transfection, holes are made in the cell membrane that allow the DNA to enter. The holes can be made by applying an electrical pulse or by adding chemicals to the cells. Once inside the cell, the gene construct may enter the nucleus and incorporate into the cell’s genome.
Step 5. Selecting for transgene positive cells
After transfection, an antibiotic is added to select the bovine cells that have incorporated the gene construct. Transgenic bovine cells will survive treatment with an antibiotic, because they contain an antibiotic resistance gene making them resistant to the antibiotic. Cells without the gene construct will have no resistance to the antibiotic and will die. In addition to antibiotic selection, polymerase chain reaction (PCR) is used to check that the bovine cell contains the transgene.
Step 6. Making a transgenic embryo using nuclear transfer
Nuclear transfer is used to create a whole animal from a single transgenic bovine cell.
The transgenic bovine cell is fused with a bovine oocyte that has had its chromosomes removed (called an enucleated oocyte). An electrical pulse is applied to help fuse the cells. Once fused with the oocyte, the transgenic cell’s chromosomes are reprogrammed to direct development into an embryo. After 7 days, the transgenic embryo will have about 150 cells and can be transferred into a recipient cow for further development to term.
Step 7. Confirming the cow is transgenic
If the embryo develops to full term, after 9 months, the cow will give birth to a calf. To confirm that the calf is transgenic, scientists can check using:
- PCR to determine the presence or absence of the transgene
- quantitative PCR (q-PCR) to determine the number of copies of the transgene
- fluorescent in situ hybridisation (FISH) to visualise where the transgene is in the chromosome and whether the transgene has integrated into more than one chromosome.
When the calf is lactating (either after being induced to lactate or after having its own progeny), its milk is checked to determine if the transgenic protein is being expressed
- 24 February 2010