Lecture 2 - Organisation of genomes

Question 1

How are bacterial genomes often arranged?

Answer 1

in operons allowing coordinated expression

• operons are often polycistronic, meaning that a single mRNA transcribed from a single promoter may contain multiple genes (terminated by transcriptional terminator)
• genes within an operon usually have a related function e.g. all the genes required for histadine biosynthesis are found in one operon

Question 2

What are the features of gene organisation on the E.coli genome?

Answer 2

• as is common for bacterial genomes, only one DNA strand is used at any location in the genome
• forward strand = 3’ to 5’
• genes encoded within operons have related functions
• short intergenic distances between the genes in operons
• sometimes, they are organised so that the stop codon (GTA) of one gene overlaps with the start codon of the next (ATG)
• estimatied 2758 different transcription unis, 795 of which are operons
• high gene density (88% DNA encodes proteins)

Question 3

What is a prophage?

Answer 3

• some temperate phage can integrate into the bacterial genome to create inactive lysogenic bacteria (prophage)
• the prophage can now potentially excise itself and start the lytic cycle whenever it wants, generally under times of stress

Question 4

Why are prophage elements important for bacterial physiology?

Answer 4

-phage often carry other genes that are not important for their own replication
-often vir factors e.g. protein toxins
-Example:
-Infection and integration of a phage like Sp-15 (lambdoid phage) can confer large phenotypic changes on the bacteria
-infection of harmless strains of S.pyogenes by a phage containing the diptheria toxin converts them to bacteria that cause scarlet fever, excises under periods of stress e.g.
take antibiotics -> inducing stress -> sublethal dosage of antibiotics causes it to turn on the transcription of all its genes very quickly ->symptoms get worse before the get better

Question 5

What is the size range of the bacterial genomes?

Answer 5

• streptomyces avermitilis MA-4680 - 9.1mb

- mycoplasma genitalium G37G-37 - 0.58mb

Question 6

What are the features of the Streptomyces coelicolor genome, what does it use its large genome for?

Answer 6

large, ~9mb

• large GC rich domains
• linear chromosome

For:
Multicellular development
-colonies can develop so that they can form arial hyphae and some cells can differentiate into spores
-contain over 20 large gene clusters for making antibiotics and other secondary metabolites
Soil dwelling
-Soil - nutritionally, biologyically and physically complex and variable environment
-expansion of the genome for regulation to sense and adapt to the environment- e.g. 65 sigma factors and over 50 two-componant systems
-degradation of extracellular nutrients

Question 7

What are the life and genomic features of Buchnera aphidicola?

Answer 7

• obligate intracellular symbiont of the pea aphid
• cells localised within specialised insect cells called mycetoctyes or bacteriocytes in the aphid body cavity
• small low GC chromosome of around 640,000bp and 600 genes
• has evolved genome reduction through its intracellular lifestyle (reductive evolution) - common ancestor with e.coli (4.6mb) 200 Mya (3.5Mb)

Question 8

How can the Buchnera aphidicola survive with so few genes?

Answer 8

Lives in a stable environment

• bacteria are alomost totally protected from environmental stresses by living inside the insect cell
• passed vertically from generation to generation, not been in the ‘outside world’ for 200mYa
• genomes have NO transcriptional regulation
• genome contains elements mainly for its symbiotic function ,which is nutritional
• bacteria provides essential amino acids to the aphid which it cannot get from its diet of plant phloem sap

Question 9

How does reductive evolution occur?

Answer 9

-by a series of deletion and inactivation of existing genes
-initial large deletions remove large regions of the genome
-followed by smaller deletions and gene inactivation
-meaning that genomes are still relatively co-linear
E.g. Buchnera aphidicola genome is a subset of the e.coli k-12 genome, although smaller, genomes are relatively co linear

Question 10

Over shorter evolutionary time what does reductive evolution result in?

Answer 10

-accumulation of pseudogenes

Question 11

Give two examples of bacteria where selective gene loss is essential for movement into certain new niches

Answer 11

Salmonella typhimurium verses typhi
Escherichia coli verses Shigella flexneri
- in both cases the later organisms have many pseudogenes, (typhi and shigella)
-it appears that inactivation of certain genes has allowed these human pathogens to exploit new niches inside the human at the expense of the host range
-inactivation of some genes may be necessary to exploit new niches e.g. Shigella and typhi human pathogens

Question 12

What is the smallest number of genes required to grow in the lab?

Answer 12

-must first define the growth conditions for growth

Scarab genomics engineered ‘Clean genome E.coli’ by deleteing 15% of the E.coli K-12 genome, all phage elements removed and it still grows fine on a minimal medium

Smallest free-living bacterium (Mycoplasma genitalium)

• 0.58Mb genome, 482 genes
• genetic studies have revealed that 100 of these genes can be mutated and still produce a viable cell
• minimal set of 382 genes

Theoretical studies suggest numbers around 250-300 genes

Question 13

How are prophage elements formed?

Answer 13

-bacterial viruses
-usually infect bacteria, copy themselves and then kill the bacteria (lytic bacteria)
HOWEVER
-some temperate phage can integrate into the bacterial genome to create lysogenic bacteria (prophage)
-the prophage can now potentially excise itself and starty the lytic cycle whenever it wants

Question 14

What is a cryptic prophage?

Answer 14

if a prophage stays in a genome for a long time it will accumulate mutations and may become inactive, ‘junk DNA’