Lecture 1: proteomics

Question 1

What is a mass spectrometer?

Answer 1

A device that measures the mass of the analytes (e.g. proteins, peptides, carbohydrates, fat, small molecule, chemicals).

Question 2

Explain the general principle of mass spectrometry (in regard to proteomics).

Answer 2

A molecule is injected into the mass spectrometer that eventually arrives at the detector. Here, the detector measures 2 parameters: mass and intensity/concentration.

Question 3

Why do we mostly measure peptides and not proteins themselves?

Answer 3

Proteins have a low resolution and poor mass accuracy (due to post-translational modifications like acetylation). Amino acids and thus peptides all have their own unique mass which can be used to identify the peptide (identify the peptides = identify the protein)

Question 4

What enzyme is used to digest proteins into proteolytic peptides? How does it work?

Answer 4

Trypsin, it cleaves the peptide bond between carboxyl group of arginine or the carboxyl group of lysine and the amino group of the adjacent amino acid.

Question 5

So easy enough you can use and identify the amino acids/peptides to determine the protein. A problem is that different amino acid sequences can have the same mass. How do we solve this problem?

Answer 5

We need to determine the sequence to identify the peptides and protein.

Question 6

So how can you determine the sequence of peptides?

Answer 6

By using tandem mass spectrometry. Here, the molecules are ionized and these ions are seperated by the first spectrometer (MS1) based on their mass-to-charge ratio (m/z). Ions of a particular m/z from MS1 are fragmented into smaller ions. These ions are then introduced intro the second spectrometer (MS2), which also separates the fragments by their m/z-ratio and detects them.

Question 7

So in tandem spectrometry a protein is digested into smaller fragments of peptides and these peptides are again fragmented into smaller fragments. How can the peptide sequence be deduced from this?

Answer 7

Each amino acid has a mass and by substracting the masses of the smaller fragments, the sequence of the peptide can be deduced.

Question 8

A sample can contain up to (or more than) 3000 proteins. A protein contains approximately 30 peptides. 90000 peptides is too complex to analyse. What is typically used to lower this sample complexity?

Answer 8

High pressure liquid chromatography (LC-MS)

Question 9

How is the complexity of a sample reduced when high pressure liquid chromatography is used?

Answer 9

By separation of peptides according to their hydrophobicity.

Question 10

Analysis of a sample during mass spectrometry can only occur in the gas phase of the sample. Name two techniques that ensure the gas phase of the sample.

Answer 10

1. Electrospray ionization
2. MALDI (not discussed)

Question 11

What is electrospray ionization?

Answer 11

The result of this technique is the formation of charged droplets in the gas phase. This is done by repeated evaporation of the sample with appliance of high voltage. This creates small droplets of charged peptides in gas phase, so that they can enter the mass spectrometer.

Question 12

A very important measurement in mass spectrometry is time of flight, What is this?

Answer 12

A mass spectrometer is composed of different chambers. You’ve got the sample inlet, the ionisation area, the acceleration area, the flight path and the ion detector. When ions are accelerated in the acceleration area they enter the flight path. Due to the difference in mass, there’s a difference in velocity. Lighter ions arrive earlier at the ion detector than heavy ions. The time ions travel in the flight path is called the time of flight.

Question 13

Why not transcriptomics only (so why are we using proteomics)?

Answer 13

Post-translational modifications are not revealed by mRNA and there’s no correlation between the amount of mRNA and protein produced.

Question 14

What are symptoms of Alzheimer’s disease?

Answer 14

Memory impairment, disorientation, personality changes, cognitive decline and eventually complete dependence.

Question 15

What mutations (probably) lay base to Alzheimer’s and what are risk factors?

Answer 15

Mutations in APP, PSEN1 and PSEN2. Risk factors are age and the apoE4 genotype.

Question 16

What’s the difference between familial AD and sporadic AD?

Answer 16

• Familial AD has mutations in APP, PSEN1 or PSEN 2 and the disease sets on early (young onset 50-60 years).
• Sporadic AD has old onset where 30-40% occurs above 80+ years.

Question 17

What is the amyloid cascade hypothesis?

Answer 17

Most importantly, accumulation and deposition of oligomeric or fibrillar amyloid-beta (Aβ) is the primary cause of Alzheimer’s. This is due to the fact that Aβ oligomers accumulate around cells, which causes cellular changes. This leads to synapse loss or neuronal death, which ultimately results in cognitive impairment.

Question 18

Alzheimer’s is a multi-factorial disease. Name different risk factors for the development of Alzheimer’s.

Answer 18

Age, infections (inflammation, innate immunity), diabetes, obesity, high blood pressure, gut microbe composition etc.

Question 19

What are three hallmarks of Alzheimer’s?

Answer 19

1. Amyloid-beta (Aβ) plaques, deposited extracellularly.
2. Neurofibrillary tau-tangles, deposited intracellularly.
3. Aβ accumulation in brain vasculature → Cerebral Amyloid Angiopathy (CAA)

Question 20

What is Cerebral Amyloid Angiopathy (CAA)?

Answer 20

Due to deposition of Aβ plaques and tau-tangles in the brain vasculature, patients with AD have a higher chance of brain haemmorhages.

Question 21

To asses the severity of Alzheimer’s disease, it is determined what Braak stage a patient is in. How is this Braak stage determined?

Answer 21

Through the amount of tau-tangles. These tangles arise first in the hippocampus and spread from this location. (This is also the reason why AD patients can’t remember anything of 10 minutes ago, but can remember things from 10 years ago, because the hippocampus is important for short-term memory).

Question 22

What is the connection between AD pathology and clinical symptoms?

Answer 22

That these two highly correlate with each other.

Question 23

Why is it actually already too late when someone gets diagnosed with Alzheimer’s ?

Answer 23

Because there’s a threshold for when clinical diagnosis is possible, but before this threshold AD pathology has already developed. This can also be seen in this picture.

Question 24

The following questions are about a proteomics analysis of CA1 and the subiculum regions of the hippocampus from human postmortem brains of AD patients and controls. What was the goal of this study?

Answer 24

• To get insights in the disease mechanisms
• To identify potential early biomarkers and drug targets for diagnosis and treatment of AD

Question 25

What was very important in this proteomics study of CA1 and the subiculum of the hippocampus?

Answer 25

Case selection. The selection was based on: no secondary disease, no vessel deviations, gliosis conform to disease stage, symptoms in accordance to pathology etc.

Question 26

This is a picture of isolated CA1 and subiculum regions from the hippocampus. What is seen here?

Answer 26

There are clear differences in the tissue of the hippocampus, the tissue that is deviant is outlined. This is also the tissue that you will isolate to analyse in a spectrometer.

Question 27

The experimental setup of this proteomic analysis of CA1 and the subiculum of the hippocampus is composed of 4 steps. What are these steps?

Answer 27

1. Isolation of CA1 and subiculum of hipoocampus by lasercapture microdissection
2. Performing SDS-PAGE on the isolated tissue
3. Proteins in-gel digested by trypsin
4. Liquid Chromatography with tandem mass spectrometry (LC-MS/MS)

Question 28

What is seen in control and AD patients in regard to tau- and GFAP levels?

Answer 28

The amount of tau-tangles and GFAP (important in astrocytes) increases with Braak stage.

Question 29

What does this figure conclude in regard to Alzheimer’s and gene activation?

Answer 29

That in certain genes/proteins there’s a turnover → in early Braak stage one group of genes is inactive while other genes are active. In progression to later Braak stages, these two groups turn around, where the first is activated and the other group of genes are inactivated.

Question 30

Study these graphs and choose and explain two graphs that display potential biomarkers.

Answer 30

Graphs E and H are the most interesting. In graph E you can see that all microtubule-associated proteins stay at a stable level during Braak stages, but only one increases in the development of AD. This is exactly the same for graph H where all ionotropic glutamate receptors stay stable, except one which increases.

Question 31

What can be concluded from this figure where they isolated tissue from control, AD and AD+CAA?

Answer 31

Certain proteins are only present when a patients has AD+CAA. For example: NDP and COL6A2 are only present in patients with AD+CAA.

Question 32

Besides Aβ plaques, tau-tangles and Cerebral Amyloid Angiopathy (CAA), what other pathology can occur in AD?

Answer 32

Granulavacuolar degeneration (GVD)

Question 33

What are processes that are related to proteins that are increased in granulavacuolar degeneration (GVD)?

Answer 33

Protein folding, endolysosomal function, glycolysis, microtubuli and cytoskeletal related proteins.

Question 34

What are processes that are related to proteins that are decreased in granulavacuolar degeneration (GVD)?

Answer 34

RNA processing and proteasome components

Question 35

I don’t think this is important, but name granulavacuolar degeneration (GVD) marker proteins.

Answer 35

PPIA, TOMM34, HSP70, CHMP1A, TPPP, VXN

Question 36

You can also use mice to study the effect of certain treatments. But what can you use when you are interested in human research, but cannot use human research?

Answer 36

Then you can use iPSC differentiated neurons or astrocytes.