StudySmarter: Study help & AI tools
4.5 • +22k Ratings
More than 22 Million Downloads
Free
There are about 3 billion nucleotides in human DNA, making it about 1.8 meters (5 feet) long! Finding a genetic mutation or a specific allele would be like looking for a needle in a haystack. However, thanks to scientists, there are easy ways for detecting specific mutations in one’s DNA. This article explores DNA and the methodology and applications of DNA hybridisation.
Explore our app and discover over 50 million learning materials for free.
Lerne mit deinen Freunden und bleibe auf dem richtigen Kurs mit deinen persönlichen Lernstatistiken
Jetzt kostenlos anmeldenNie wieder prokastinieren mit unseren Lernerinnerungen.
Jetzt kostenlos anmeldenThere are about 3 billion nucleotides in human DNA, making it about 1.8 meters (5 feet) long! Finding a genetic mutation or a specific allele would be like looking for a needle in a haystack. However, thanks to scientists, there are easy ways for detecting specific mutations in one’s DNA. This article explores DNA and the methodology and applications of DNA hybridisation.
DNA probes are short pieces of single-stranded DNA labelled to be easily identified. The probes can be designed to be complementary to a specific allele or mutation so that they can specifically bind to those sequences.
Two types of DNA probes are commonly used. They are:
DNA hybridisation describes the combination of a section of DNA with a single-stranded piece of DNA that contains complementary sequences.
DNA RNA hybridisation describes the combination of a section of RNA with a single-stranded piece of DNA that contains complementary sequences.
In the context of this article, the single-stranded piece of DNA is the DNA probe, and the section of DNA or RNA is a particular allele.
A variant of a gene is called an allele.
For the probe to bind to the complementary sequence of the specific allele, the double-stranded DNA needs to be separated. Heating the DNA sample denatures the DNA molecules and separates the two strands by breaking the hydrogen bonds between them.
Then the separated DNA strands would be mixed with the probes, and the temperature would be lowered, allowing for hydrogen bonds to be formed (anneal) between complementary DNA strands. Although most of the DNA strands would pair up with their original complementary strand, some strands would bind to the probes. This binding process is referred to as DNA hybridisation.
DNA probes and DNA hybridisation can be used to locate a specific allele. This process involves many steps:
Thanks to the work of countless scientists around the world, we now know the location and type of mutations that cause many hereditary diseases. DNA hybridisation and DNA probes can be used to screen individuals for specific hereditary conditions.
Multiple genetic mutations can be simultaneously investigated by fixing multiple DNA probes in an array on a glass slide and then adding the donor DNA to the array. Any complementary DNA sequences, if present, would then bind to their corresponding probe.
Genetic screening can detect oncogenes (genes that increase the likelihood of developing cancer). There are two types of oncogenes, tumour suppressor genes and proto-oncogenes.
Tumour suppressor genes code for proteins that act as breaks in the cell cycle and stop potentially cancerous cells from proliferating.
Proto-oncogenes code for proteins that accelerate the cell cycle and promote cell proliferation.
Therefore, any mutation that inactivates tumour suppressor genes or increases the activity of proto-oncogenes can result in uncontrolled cell division and lead to the development of cancer.
The presence of mutations in these proto-oncogenes can be detected by genetic screening. This would allow the individual with the mutation to make an informed decision about their lifestyle. For instance, they would be able to lower the risk of developing cancer by eating healthier and avoiding mutagenic substances such as cigarette smoke.
Mutagens are chemicals or anything that can create a mutation in the DNA.
People can also undergo regular check-ups to detect cancer early and improve the chances of successful treatment.
Another advantage of genetic screening is personalised medicine. It allows doctors to treat patients based on their genotype. For instance, drug A may be more effective in treating a condition in one patient but not another patient with a different genotype. Another drug can then be used for the other patient that provides maximum efficacy in their treatment.
Knowing the patients’ genotypes allows doctors and pharmacists to prescribe the exact dose of a specific medicine to produce the desired outcome on the patients’ treatment plan. This would save money and prevent any unnecessary harm and side effects that some medications may have.
The liver contains enzymes that metabolise and remove drugs such as painkillers. Different individuals express varying levels of these enzymes depending on their genotype. Therefore, some individuals with higher levels of liver enzymes may need more painkillers than others. Knowing one’s genotype allows for a safer and more effective prescription of painkillers.
Vitamin E is known to lower the risk of cardiovascular disease in diabetic individuals with a certain genotype. However, vitamin E increases the risk of cardiovascular diseases in diabetic individuals with a different genotype. Therefore, knowing one’s genotype can allow for a better informed and safer prescription of vitamin E supplements.
Genetic counselling is a special form of social work. It provides advice and information to people, helping them make personal decisions about themselves and their children. Based on family history of hereditary conditions and genetic screening, genetic counselling can inform couples about their children’s chances of having a disease.
Here is some information to refresh your memory; alleles are usually either dominant or recessive. Suppose an individual is heterozygous for the dominant allele (i.e. has the dominant allele on one chromosome and the recessive allele on the other chromosome). In that case, they will show the dominant phenotype despite carrying the recessive allele. Only if an individual is homozygous for the recessive allele (i.e. has the recessive allele on both chromosomes) will they have the recessive phenotype.
Remember sickle cells anaemia? It is caused by a mutation in the gene coding for the beta-globin polypeptide, a subunit of haemoglobin. The mutated sickle cell allele is recessive to the wild type globin beta allele. Therefore, a heterozygous individual will not have symptoms of sickle cell anaemia.
However, if one heterozygous individual had offspring with another heterozygous individual, there would be a 25% chance that their child would be homozygous for the sickle cell allele and hence would have sickle cell anaemia. Genetic screening allows the identification of a mutated recessive allele in heterozygous individuals who have the dominant and healthy phenotype.
Counsellors would inform couples about their children’s chances of having a disease and provide further information about its emotional, psychological, medical, social and economic consequences. Based on the counsellor’s advice, couples would then choose whether or not to have children.
Despite the many advantages of genetic screening, there are some major ethical considerations around genetic counselling. Genetic counsellors face a common ethical dilemma involving genetic screening on pregnant patients. We mentioned earlier that genetic screening could determine whether one or both parents are carriers of a medical problem. Other tests can determine whether the fetus has genetic mutations that will result in birth deformities, mental disability, or physical impediments. Counsellors may find it ethical challenging if they know that their pregnant patients may decide to terminate the pregnancy over carrying a fetus to term.
Inappropriate testing is another ethical challenge that surfaced when genetic testing became increasingly prevalent. This refers to couples who seek genetic counselling and testing in the hopes of having a baby with specific characteristics that they desire. Couples can undergo testing and abort pregnancies that do not result in ideal children, or even pregnancies that result in a child of the opposite sex to the one they desired.
DNA probes are short pieces of single stranded DNA that are labelled so that they are easily identifiable.
The probes can be designed to be complementary to a specific allele or mutation so that they would be able to specifically bind to those sequences
DNA hybridisation describes the combination of a section of DNA or RNA with a single stranded piece of DNA probe that contains complementary sequences and is labelled to ease its detection.
DNA hybridisation describes the combination of a section of DNA or RNA with a single stranded piece of DNA that contains complementary sequences
In order for the probe to be able to bind to the complementary sequence of the specific allele, the double stranded DNA needs to be separated. This is done by heating the DNA sample which denatures the DNA molecules and separates the two strands by breaking the hydrogen bonds between them.
Then the separated DNA strands would be mixed with the probes and the temperature would be lowered allowing for hydrogen bonds to be formed between complementary DNA strands (anneal). Although the majority of the DNA strands would pair up with their original complementary strand, some strands would bind to the probes. This binding process is referred to as DNA hybridisation.
What is a DNA probe?
DNA probes are short pieces of single stranded DNA that are labelled so that they are easily identifiable.
What is DNA hybridisation?
DNA hybridisation describes the combination of a section of DNA or RNA with a single stranded piece of DNA probe that contains complementary sequences and is labelled to ease its detection.
Name two different types of DNA probe labelling?
Radiolabelling with radioactive phosphorous or labelling with a fluorescent dye
Why are donor DNA molecules heated before DNA hybridisation?
To break the hydrogen bonds between strands and separate the DNA strands from each other.
How is the sequenc of DNA probes designed?
By either sequencing a piece of DNA that contains the mutation or referring to genetic libraries.
How are DNA fragments amplified?
By using PCR
Already have an account? Log in
Open in AppThe first learning app that truly has everything you need to ace your exams in one place
Sign up to highlight and take notes. It’s 100% free.
Save explanations to your personalised space and access them anytime, anywhere!
Sign up with Email Sign up with AppleBy signing up, you agree to the Terms and Conditions and the Privacy Policy of StudySmarter.
Already have an account? Log in