11/12/13/14 - Organelles and their genomes Flashcards

1
Q

What is primary, secondary and tertiary endosymbiosis?

A

Primary: I prokaryote, 1 membrane

Secondary: A organism consumes another with an endosymbiont (2 membranes)

Tertiary: 3+ membranes

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2
Q

True or false, a chloroplast has only a few copies of cpDNA?

A

False, each organelle has many copies.

There is about the same amount of DNA present in organelles (combined) as the nucleus

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3
Q

Give two methods for studying organelles and their genomes with comparative genomics

A
  • compare organellar genomes to those of bacteria. Can learn about impact of endosymbiosis on the eukaryotic nuclear genome.
  • Compare organellar genomes to nuclear genomes of different species. Can tell us how organellar DNA evolves and migrates to the nucleus over shorter timescales.
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4
Q

How do you study endosymbiotic gene transfer in the lab?

Give the example with the tobacco plant

A

Experimental systems involving transgenic organisms can be used to observe EGT in real time. Can provide insight into the mechanisms and frequency of EGT.

Experiment in tobacco plant

  1. Link a gene to a “plastid-specific” promoter to confer resistance to spectinomycin
  2. Link another gene to “nucleus specific” promoter to confer resistance to kanamycin (still in plastid)
  3. Resistant to only plastid specific drug
  4. Screen for kanamycin resistance, if it grows it means that the gene has migrated to the nucleus and the nucleus-specific promoter containing gene can be expressed.
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5
Q

True or false. Endosymbiotic gene transfer takes place over different timescales

A

The mass migration of DNA from organelle to nuclear runs at a very variable rate (true!)

  • Ancient transfers (eg. during evolution from mitochondrial/plastid progenitors)
  • Somewhat recent transfers (organelles have different size genomes in different species)
  • Very recent transfer (usually giving rise to non-functional DNA fragments continuously - eg. in tobacco)
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6
Q

How widespread is endosymbiotic gene transfer?

A

Very!

The mitochondrial genome has become very small in most organisms (sometimes to nothing), the plastid genome is even smaller (sometimes to nothing as well).

Both proteomes are usually under 1000 proteins!

The proteins that both organelles need are provided by the nuclear genome.

If the organelle provides any genes, it is quasi-autonomous.

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7
Q

Describe the genomic ‘footprint’ of endosymbiosis in Arabidopsis thaliana

A
  • Almost 25% of the nuclear genome is from the cyanobacterial progenitor of the plastid. So there is a huge footprint because of extensive EGT.
  • Nucleus encoded cyanobacterium derived proteins are targeted to different subcellular locations (not just the plastid)
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8
Q

Define EGT

A

Endosymbiotic gene transfer - The process by which fragments of endosymbiont/organelle DNA ends up in the nuclear genome.

Doesn’t need to be intact genes!

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9
Q

Define NORGs

A

Nuclear integrant of organellar DNA

Includes:

  • NUMTs
  • NUPTs

We can say very confidently that these fragments come from their respective organelles.

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10
Q

Define NUMTs

A

Nuclear mitochondrial DNA

  • Mitochondrial DNA fragments integrated into the nuclear genome
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11
Q

Define NUPTs

A

Nuclear plastid DNA

- Plastid DNA fragments integrated into the nuclear genome.

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12
Q

Define NUNMs

A

Nuclear nucleomorph DNA
- Fragments of DNA from nucleomorph genomes integrated into the nuclear genome (limited to single celled algae with nucleomorphs obviously)

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13
Q

True or false? The total amount and density of NUMTs and NUPTs varies a lot!

A

True!

The total amount varies between mitochondria and plastids in the same organism!

Eg. Arabidopsis has lots of NUMTs but not nearly so many NUPTs

The amount can even vary among organelles in an organism.

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14
Q

Describe how the Domestic Cat provides an example of NUMTs

A
  • An 8 kb NUMT migrated to the nuclear genome and hybridized with a nuclear chromosome and duplicated massively there as a tandem repeat
  • The spread is mediated by recombination
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15
Q

In humans, did NUMTs arise before or after the divergence of humans and chimpanzees? Why is it hard to answer this question?

A

Before AND after

It is not clear how many human NUMTs represent unique NUMT transposition/transfer events vs. duplications of previous transposition events.

Because of this, there is lots of NUMT variation even among individuals!

It is hard to count NUMTs because they can jump into the genome and then jump around them.

NUMTs also disappear fairly quickly, they acquire mutations and deletions at a rate similar to pseudogenes. So they are only detectable for a short amount of time.

When there is a lot of EGT, it is hard to determine if you are just reading background noise (from lysed organelles) or true nuclear genes.

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16
Q

True or false, NUMTs can cause disease. Why or why not?

A

True

eg. putting a premature stop codon into an important nuclear gene will result in a nonfunctional protein.

This can be caused by DNA damage (eg from radiation), making the genome more accepting of foreign elements/recombination. Spontaneously. Or the diseases can be inherited if the insertion occurs in the germ line.

17
Q

True or false, NUMTs can go on to become active elements of the nuclear genome?

A

True.

In Bigelowiella natans, a NUMT inserted into a gene and became an active intron. Because it is spliced out, no harm done!

18
Q

Is there a correlation between number of organelles in a cell and endosymbiotic gene transfer prevalence?

A

Yes.

More organelles = more transfer events

Organelle lysis is the main mechanism for DNA transfer from organelle to nucleus.

19
Q

How much DNA is usually transferred in endosymbiotic gene transfer?

A

Any fragments can be transferred in principle. From ten bp fragments to an entire organellar genome.

20
Q

How is organellar DNA integrated with nuclear DNA? Is this random and can only DNA be integrated?

A

NUMTs and NUPTs are incorporated non-homologously.

Non-homologous end joining at sites of double-strand break (DSB) repair. Integration appear to be non-random (eg. into A/T rich regions more)

cDNA from organellar RNA can also be integrated

Summary: DNA damage followed by DSB repair with organellar DNA

21
Q

What is the fate of transferred DNA (and the donor DNA in the organelle) after EGT?

A
  • Majority of EGTs are non-functional: they quickly become pseudogenes and disappear due to mutations
  • Donor DNA continues to exist in the organelle OR if the gene is successful in the nucleus, it will be deleted from the organellar genome.
22
Q

Giv e three qualities of a good potentiation insertion site for EGT

A
  • A+T rich
  • Highly bendable
  • Open chromatin
23
Q

How are the products of genes transferred from the organelle to the nucleus imported to the organelle?

A
  • N-terminal signal sequences (transit peptides) bind with receptors on surface of organelle
  • Protein machinery (TOMs/TIMs/TOCs/TICs) mediate translocation of the protein
  • Transit peptide removed once protein is inside the organelle
24
Q

Name the translocons of mitochondria and chloroplasts?

A

Mitochondria: TOMs and TIMs

Chloroplasts: TOCs and TICs

25
Q

What three elements are needed for a NUPT or NUMT to provide proteins for their organelle?

A
  • Promoter
  • Transit peptide
  • Terminator
26
Q

When does an endosymbiont become an organelle?

A

When both endosymbiotic gene transfer AND protein import can take place (ie. a dedicated protein import apparatus is in place.

27
Q

Is the nucleus a membrane bound organelle?

A

No, because the nuclear envelope is continuous with the endoplasmic reticulum.

28
Q

Describe the case of Paulinella chromatophora and how its chromatophores relate to plastids

A

It is a single celled eukaryote with two sausage like chromatophores, which divide synchronously with the host cell. The host and chromatophores cannot grow apart from one another.

  • Chromatophores evolved from cyanobacteria independent of plastids
  • The chromatophore genome appears to be undergoing reduction (lots of pseudogenes, which are uncommon in prokaryotes)
  • Plastids are about a billion years old, this endosymbiosis is only about 60 million years old
29
Q

Is the chromatophore of paulinella chromatophora an endosymbiont or an organelle?

A

Organelle

  • There is EGT occuring, with genes of chromatophore origin in the host nuclear genome
  • Targeting of nucleus encoded proteins to the chromatophore has been observed

So EGT + protein import satisfies organelle requirements

30
Q

Is Buchnera an endosymbiont of aphids? Or organelles?

A

EGT has taken place but there is no FUNCTIONAL gene transfer or protein import taking place: endosymbiont

Though, there is one gene (RlpA4) which encodes a lytic transglycosylase with an N-terminal signal peptide to target to the ‘endosymbiont/organelle’

Blurry distinction between endosymbiont and organelle in this case. Perhaps organelle in the making.

31
Q

How do transferred genes acquire gene expression and targeting elements?

Give four methods

A

They acquire them de novo, but they can also acquire them from pre-existing genes:

  • De novo acquisition
  • Insertion into duplicated copies of other genes (steals elements from a non-necessary gene copy)
  • Insertion into a tandem duplication (one of the two is dispensable)
  • Insertion into an intron, with co expression by alternative splicing.
32
Q

Describe the key features of the gene-transfer ratchet

A
  • EGT is unidirectional
  • EGT is accidental and inevitable
  • Intact genes on fragments will sometimes (rarely) be expressed and even more rarely inserted downstream of a region encoding a N-terminal targeting sequence, allowing protein import.
  • If the nuclear copy of the gene is lost, evolution can try again
  • If gene B is lost from organellar genome, it is lost forever from that genome and the nuclear copy becomes essential for survival.

After time, the nuclear genome will ultimately incorporate all organellar genes that can potentially function there

33
Q

Give three hypothesis for the retention of organellar genomes

A
  • Hydrophobicity hypothesis: organellar genome coded proteins are hydrophobic, making them hard to import across the membranes of the organelle (very true for mitochondria, less true for plastids)
  • Redox regulation hypothesis: Electron transport proteins must be quickly directedly regulated by redox state of mitochondria, in cases where the mitochondrial genome has disappeared, the electron transport chain is no longer used.
  • Genetic code disparity hypothesis: There is always at least one disparity between a cell and the organellar genome’s genetic code (doesn’t hold up for all cases)
34
Q

What are the two main types of plastids?

A

Primary plastids: evolved directly from cyanobacteria and surrounded by two membranes.

Secondary plastids: Acquired indirectly from primary plastid-bearing algae, surrounded by three or four membranes.