Title: Chapter 8: Bacterial Genetics
1Chapter 8Bacterial Genetics
2Important Point
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3Bacterial Genetics
- Acquiring genes through gene transfer provides
new genetic information to microorganisms, which
may allow them to survive changing environments. - The major source of variation within a bacterial
species is mutation. - In mutations, usually only a single gene changes
at any one time. - In contrast, gene transfer results in many genes
being transferred simultaneously, giving the
recipient cell much more additional genetic
information.
4Bacterial Genetics Overview
- Most bacteria are haploid which means that there
is no such thing as dominance-recessive
relationships among bacterial alleles. - Bacteria dont have sex in the animal/plant sense
of sex (i.e., mating followed by recombination of
whole genomes). - Instead, bacteria acquire DNA from other bacteria
through three distinct mechanisms - Transformation
- Transduction
- Conjugation
- This DNA may or may not then recombine into the
recipients genome. - We use phrases like Lateral or Horizontal
Gene Transfer to describe these sexual
interactions. - Bacterial DNA is also subject to mutation, damage
(not the same thing as mutation), and natural
selection.
5Mutation Terms Concepts
- Wild Type refers to the microorganism as isolated
from the wild. - A mutated microorganism that has lost a metabolic
function, particularly an ability to synthesize a
specific growth factor, is called an Auxotroph. - The wild-type parent to an auxotroph is called a
Prototroph. - A Mutation is found in a gene a mutant is an
organism harboring a Mutation. - We designate mutant phenotypes using three-letter
abbreviations the phenotype of a
tryptophan-requiring auxotroph would be described
as Trp-. - A bacterium that has mutated to resistance to an
antibiotic (or other substance) is given the
superscript R thus, the phenotype ampicillin
resistance is indicated as AmpR. - Mutants can be spontaneous or induced by a
Mutagen an agent that causes DNA to mutate.
6Types of Mutations
- Base Substitution
- Point mutation single base is substituted.
- Missense mutation base change changes single
amino acid to different amino acid. - Nonsense mutation base change changes single
amino acid to stop codon. - Null or Knockout mutation mutation that totally
inactivates a gene. - Deletion or insertion mutation change in number
of bases making up a gene. - Frameshift mutation insertion or deletion of
something other than multiples of three bases. - Frameshifts typically radically change downstream
codons, generating stop codons, and typically
knocking out gene function. - Reversion mutation mutated change back to that
of wild type.
7Rates of Mutation
- The mutation rate of different genes usually
varies between 10-4 and 10-12 mutations per cell
division (essentially equivalent to per cell). - 10-4 one in 10,000 10-12 one in one
trillion. - To calculate the probability of two independent
mutations we multiple the two mutation rates. - Thus, if streptomycin resistance occurs at a rate
of 10-6 mutations per cell division and the rate
of mutation to resistance to penicillin is 10-8
then the rate of mutation to both antibiotics is
10-6 10-8 10-14 (note that the exponents are
added). - That is, we would have to have a population of
one-hundred trillion cells to have one double
mutant, which even for bacteria is a lot of
cells. - This is the basis for Combination Therapy, e.g.,
the use of more than one chemotherapeutic against
tuberculosis, HIV, cancer, etc. - The odds of sufficiently multiply resistant
mutants drops with each new chemotherapeutic
added to the mix.
8Direct Selection for Mutants
9Indirect Selection Replica Plating
10Indirect SelectionPenicillin Enrichment
11Indirect SelectionIsolation of ts Mutants
This is one example of isolation of mutants
carrying conditionally lethal mutations found in
essential genes.
12Ames Salmonella Test
13DNA-Mediated Transformation
Note that DNA is taken up naked from the
environment.
14DNA-Mediated Transformation
15Original Transformation Exp.F. Griffith (1928)
using pneumococci
16Artificial Competenceby Electroporation
Competence denotes the ability to take up DNA
naked from the environment.
Most bacteria are not naturally competent but
many can be made artificially so.
Artificially induced competence is very important
to gene cloning.
17Generalized Transduction
Bacteriophages are viruses that only infect (and
can kill) bacteria.
18Generalized Transduction
19Conjugation Sex or F Pilus
20Conjugation F Plasmid Transfer
21F and Other Plasmids
- F plasmids encode genes that allow both their
replication and transfer. - They are thus known as Self-Transmissible
Plasmids. - There are other plasmids that can take advantage
of conjugation but dont encode the the necessary
genes. These are non-self transmissible plasmids. - Transduction is also capable of transferring
smaller plasmids. - R plasmids are named not for their mode of
transmission but instead for the resistance genes
that they encode such as to antibiotics. - Some plasmids are present in bacteria in low copy
numbers (1 or 2/bacterium) whereas other plasmids
are present in high copy numbers (such
100s/bact.). - Plasmids, R and otherwise, can have very wide
host ranges allowing easy transfer of already
evolved genes between bacterial species.
22Self-Transmissible R Plasmid
Note multiple resistance genes.
Resistance Transfer Factor (conjugation genes)
23Transfer of non-R Virulence Factors
- Genes that can make bacteria more virulent (able
to cause disease) are called Virulence Factor
genes. - Virulence factors include fimbriae that allow
attachment to host tissues, exotoxins, etc. - Virulence factor genes may be transferred by
transformation, transduction, or conjugation. - Virulence factor genes tend to congregate on
bacterial chromosomes in regions known as
Pathogenicity Islands. - New bacterial pathogens can emerge via the uptake
of entire pathogenicity islands transferred
intact from unrelated bacteria.
24Transfer Protection R-M Systems
- Not all incoming DNA is necessarily good for the
receiving bacterium (i.e., DNA can be parasitic). - Bacteria employ Restriction Enzymes to protect
themselves from the foreign DNA. - Restriction enzymes recognize specific,
palindromic (same spelling backward and forward)
DNA sequences of 4 to 8 base pairs in length that
are known as Recognition Sequences. - Bacteria also employ Modification Enzymes that
modify DNA to protect it from Restriction
Enzymes. - Together these are called Restriction-Modification
Systems. - Restriction enzymes are crucial components of
genetic engineering.
25Restriction Endonuclease Action
26Restriction Endonuclease Action
Note in particular that DNA is cut at palindromic
regions.
27DNA Modification RE Protection
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