Functional Genomics

Question 1

What is functional genomics

Answer 1

Finding gene functions and interactions through whole genome at once

Question 2

What do microarrays measure

Answer 2

Hybridisation between nucleic acids and exploits their comp base pairing mechanism

Question 3

What are attached to microarray which bind complementary dna

Answer 3

Probes which fluoresce after binding

Question 4

What would probes be designed for to test methylation using micro arrays

Answer 4

Cpg islands. Probes would bind and it would detect areas of methylation for computer analysis

Question 5

How would you find a protein bs using microarrays

Answer 5

Via chip first then purify dna from the protein and probe the dna that was bound with protein and sequence it

Question 6

What would be probed to test gene expression via microarrays

Answer 6

Mrna would be RT into cDNA and probes designed complementary to it

Question 7

How can you find snps using microarrays

Answer 7

SNPs would reduce levels of hybridisation which can be measured

Question 8

Why is next gen sequencing used instead of microarrays

Answer 8

Less noisy data (measures sequence directly not via hybridisation)

Single base pair resolution

Cheaper

Detect rarer mrnas

Question 9

What is next gene sequencing / high throughput sequencing most used technique

Answer 9

Illumina sequencing

Question 10

Explain illumina sequencing

Answer 10

A dna sample obtained and fragmented

and attached to adaptors. These adapters allow binding to a flow cell

Bridge PCR then causes amplification of the same dna sample many times across flow cell

A primer attaches to allow labelled nucleotides to be added to the comp dna fragment

The nucleotides fluoresce diff colours and terminate/block extension so you detect which one was added at which time point for sequencing

Question 11

What is PCR of the same dna fragment called in illumina

Answer 11

Solid phase bridge PCR - uses adaptors

Question 12

What are the same dna fragments amplified called in illumina

Answer 12

Clonal clusters

Question 13

Is termination via labelled nucleotides reversible

Answer 13

Yes. After every cycle you can add another base for sequencing

Question 14

How is rna sequencing done via illumina to detect gene expression

Answer 14

Mrna is pulled out of a sample using its poly A tail which attached to a dT magnetic bead which pulls it from the sample

Mrna is then fragmented

RT into cDNA and copied for ds dna

Fragmented ds dna attached to adaptors for solid phase bridge PCR on flow cell

Question 15

How can you tell how much mrna was in sample at start of rna sequencing

Answer 15

It is proportional to the amount of sequence data present

Question 16

What is an issue with rna seq via illumina

Answer 16

A lot of data needs expert skills

Question 17

What is ATAC sequencing

Answer 17

Measures openness / confirmation of dna

If it’s chromatin bound via histones transposase enzyme won’t be able to cut it

If it’s open it is fragmented = shows where there are high exp levels

Question 18

What is bisulphite sequencing used for

Answer 18

Detect methylation levels

Question 19

How does bisulphite sequencing work

Answer 19

Bisulphite will usually deaminate C to T in dna but this is inhibited if the c is methylated

After sequencing you can detect where methylation is because c wasn’t deaminated

Tells you where there are levels of low expression