Faculty of Sciences and Technology of University of Coimbra Biochemistry Master Metabolism 2011/2012
Compartmentation of glial and neural metabolism in Alzheimer’s Disease
Daniela Rodrigues José Pedro Mendes Lídia Grilo Filipa Moreira
3 years of work: Separate the individuals
Quantitive analysis of the metabolites present in hipocamppus
Differences of glial and neuronal metabolism
• Cognitive/behavior tests; • MRI, (FDG)-PET; • CFS expression of protein tau and βamyloid.
• 1H-MRS (single-voxel) • Glutamate/Glutamine; • Lactate; • GABA; • N-Acetyl-Aspartate
• Administration of [U13C] glucose and [2-13C] acetate • Metabolite fluxes • Steady state
early
Controls
vs
AD Patients
moderate
advanced 25 participants in each group – 100 in total
Aims Develop a protocol to discriminate AD patients in three states of the disease development, using several criteria’s: brain morphology, cognitive behavior, biochemical metabolism and proteins levels;
Characterization and quantification of the hippocampus metabolism in patients with AD in every state (early, moderate and advanced) using H-MRS technique.
Compartmentation of glial and neuronal metabolism
Alzheimer’ Disease (AD)
• Degenerative Disease • No cure • Treatment of the symptoms
worldwide scenario (estimated): 2010 – 35.6 million people 2030 – 65.7 million people 2050 – 115.4 million people.
Decreased schooling
Normally, appears in individual > 65 years
Major risk to have AD
Each patient suffers from Alzheimer's disease unique way, but there are commonalities
Memory
Fig.1 – Brain imaging of a healthy individual (left) and Alzheimer’ patient (right).
Cell morphology characteristics: Neural loss
Loss of connections between neurons Senil Plaques Neurofibrillary Tangle
Fig. 2 – Neural alterations in Alzheimer Disease
Stages / Symptoms • • • • • • •
1st Stage
Lost short term memory; Loss of attention; Apathy; Some disorientation of time and space; Only performs simple tasks; Difficulty in recognizing and identifying objects (agnosia) Difficulty in execution of movements (apraxia).
2nd Stage
• • • • • •
Difficulty of independence; Missing remembering vocabulary; Emotional instability; Irritability; Aggressiveness; Illusions
3rd Stage
• • • • • •
Completely dependent on people to perform tasks; Loss of speech; Aggressiveness; Apathy extreme; Tiredness; Loss of mobility.
Task 1- Diagnosis and prognosis of AD 1.1 AD diagnosis using Cognitive – behavior tests We will perform 3 types of tests:
• Mini–mental state examination (MMSE) • Alzheimer's disease Assessment Scale – Cognitive Subscale (ADAS-Cog) • Clinical Dementia Rating Scale Sum of Boxes (CDR-SB) • Caucasians • 60-80 years of age; • same level of education (less than 8 years) • Mediterranean diet during their life • Absence of genetical factors that leads to AD
Task 1- Diagnosis and prognosis of AD 1.1.1 Mini–mental state examination • Questionnaire test used to screen dementia and cognitive impairment • Simple questions and problems in a number of areas:
the time and place of the test repeating lists of words arithmetic such as the serial sevens language use and comprehension basic motor skills
• It can be used to follow the course of cognitive changes in an individual over time.
decline per year: - less than 2 points - slow progressors, - 2 to 4 points - intermediate progressors - more than or equal to 5 points - rapid progressors
Task 1- Diagnosis and prognosis of AD 1.1.2. Alzheimer's disease Assessment Scale - Cognitive Subscale (ADAS-Cog)
•
Specifically designed to evaluate the severity of cognitive and non-cognitive behavioral dysfunctions characteristic of persons with AD
more thorough than MMSE considered the best brief exam for the study of language and memory skills
ADAS Cognitive domains evaluated: Cognitive
(ADAS-Cog)
NonCognitive
memory (50%) language (28%) praxis (14%) command understanding (8%)
The ADAS-Cog scores clearly distinguish clinically diagnosed AD patients from non-dementia control subjects! [1].
Task 1- Diagnosis and prognosis of AD 1.1.3. Clinical Dementia Rating Scale Sum of Boxes (CDR-SB)
•
Allow as to asess global performance of the participant patient interview mental status examination an interview of a collateral source
Six cognitive domains or boxes:
CDR is credited with being able to discern very mild impairments.
memory orientation judgment/ problem solving community affairs home and hobbies personal care
Table I - Score ranges to MMSE, ADAS-Cog and CDR-SB test corresponding to normal participants and AD patients in an early, moderate and advanced stage.
Test / Group MMSE ADAS-Cog CDR-SB
Controls 25-30 ≤24 0-3
early 21-24 25-49 4-8
moderate 10-20 50-59 9-13
advanced ≤9 60-70 14-18
Task 1- Diagnosis and prognosis of AD 1.2. MRI and fluorodeoxyglucose (FDG)-PET brain analysis AD patients exhibit: Regional cerebral atrophy - MRI Hypometabolism - (FDG)-PET MRI morphometry: - hippocampal volume - entorhinal and retrospenial cortical thickness.
FDG-PET: - entorhinal, retrosplenial and lateral orbitofrontal metabolism.
MRI can be used to quantify regional atrophy distinguishing early and later preclinical stages of AD.
Fig .3- The regions of interest used: 1) hippocampus, 2) entorhinal, 3) parahippocampal, 4) retrosplenial, 5) precuneus, 6) inferior parietal, 7) supramarginal, 8) middle temporal, 9) lateral orbitofrontal and 10) medial orbitofrontal cortices [1].
Task 1- Diagnosis and prognosis of AD 1.2. MRI and fluorodeoxyglucose (FDG)-PET brain analysis Experimental protocol: Subjects will be scanned after a 4 hour fast (water only). Plasma glucose has to be ≤ 180 mg/dL for FDG to be injected. Dosage ranges from 0.1 to 0.2 mCi per kg of body weight. Imaging begins at 30 min post injection The scan will be acquired as six 5-min frames. Fig. 4Typical positron emission tomography (PET) facility
The distribution of 18F-FDG is a good reflection of the distribution of glucose uptake
PET scan of the brain
2-Deoxy-2-fluoro-D-glucose Or Fluorodeoxyglucose (18F)
Task 1- Diagnosis and prognosis of AD 1.3. CFS expression of protein tau and β-amyloid Biochemical analysis of the CSF to establish the levels on the 3 stages of AD of:
• Aβ42 • t-tau • p-tau Immunoassay method - CSF samples will be obtained by lumbar puncture - ratio of t-tau/Aβ42 and p-tau /Aβ42 will be calculated
High CSF tau levels probably reflect axonal degeneration In AD, there are high levels of p-tau, consequence of the self-assembly of tangles of paired helical filaments and straight filaments.
Fig 5. Representation of amyloid plaques formation.
Controls
AD patients
Aβ42
200 pg/mL
140 pg/mL
T-tau
70 pg/mL
125 pg/mL
P-tau
25 pg/mL
45 pg/mL
T-tau/Aβ42
0,20
1
P-tau/Aβ42
0,15
0,36
Task 2- Quantitive analysis of brain metabolites 1H-MRS
single voxel
N-acetyl-aspartate compounds
Glutamate/Glutamine; GABA;
Lactate.
N-Acetyl-Aspartate: activation of NMDA (ionotropic receptor). Marker for mitochondrial functions and loss of neuronal cells;
Lactate: barley used by neurons and glial cells, increase levels in AD indicates; GABA- inhibitory neurotransmitter. GABAergic neurons synthesize GABA by the descarboxylation of glutamate via Glutamate descaboxylase
Task 2- Quantitive analysis of brain metabolites Deficiency in glutamate/glutamine cycle
Equal changes observed in AD
See glutamate levels by H-MRS
Fig. 6 - Conversion of glutamate to glutamine by GS in the synaptic cleft. The glutamine is exported to the neuron reconverted into glutamate
Task 3 – 13C MRS measure of glial and neural metabolism Advanced technique that allows non-invasive in vivo evaluation of metabolite concentrations 13C MRS is feasible on a clinical 1.5 T MR scanner Specific diagnostic information - value in neurological research Step 1 Step 2 Step 3 Step 4
• Intravenous administration of [U-13C]glucose • Intravenous administration of [2-13C]acetate • Determination of relative metabolic fluxes • Evaluation of Steady-State conditions
• Evaluation/Comparation of metabolites between controls and AD patients Step 5
Step 1- [U-13C]Glucose
Fig. 7 Metabolism of [U-13C] glucose administred to all individuals, where labeled pyruvate is converted in acetly-CoA by pyruvate dehydrogenase.
Fig. 8 Metabolism of [U-13C] glucose administred to all individuals, where labeled pyruvate is converted to oxaloacetate by pyruvate carboxylase. [5]
Step 2- [2-13C]acetate
Fig. 9 Pathway of [2-13C] acetate in glial and neural cells. [6]
Step3-Determination of relative metabolic fluxes Obtained 13C isotopomer data
Tca CAL Program
Fractional contributions to acetyl-CoA in SS
Decreased requirement of astrocytes to replenish oxaloacetate in the TCA cycle Lower flux through astrocytic PC
The clearance of GABA by astrocytes Conversion into succinate TCA cycle
Step4: Evaluation of Steady-State Condition [U-13C]glucose and [2-13C]acetate are oxidized
Glutamate C4 becomes enriched in the 1st turn of the TCA cycle
C3 and C2 isotopomers become enriched in the following TCA turns
The glutamate C3/C4 enrichment ratio used to evaluate metabolic Steady-State (7.5 h after infusion)
Possible results from 13C MRS In normal : Glucose carbons are transported to the neuron entering the TCA cycle: - Glu4 (round 1) - Glu2 (round 2) - CO2 (round 3). - Glutamate returns carbon to the glia after neurotransmission for conversion to glutamine (Gln4 and Gln2). In AD: - All neuronal processes are systemically reduced to half - Glial glucose enriches glutamine before glutamate - Excess glucose in AD is metabolized only as far as lactate.
Fig. 10 Traffic of glutamate between neurons and astrocytes in normal and AD individuals.
Budget Reagents [U- 13C] Glucose
29 000 €
[2-13C] acetate
20 300 €
MRI
36 000 €
PET
24 000 €
2-Deoxy-2-fluoro-Dglucose
500 €
1H-MRS
15 000 €
13C-MRS
15 000 €
Other material
40 000 €
TOTAL
179 800 €
[U- 13C] Glucose
145€/0,5g (Cambridge Isotope Lab)
[2-13C] acetate
203.50€ /g (SigmaAldrich)
2-Deoxy-2-fluoro-Dglucose
813.00/100mg (SigmaAldrich)
We expect to have the support of HUC people! (for free)
References 1. 2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14.
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