Ectosomes, New Biomarkers of Tau Pathology?

Recruiting

• Conditions: Alzheimer Disease
• Interventions: Diagnostic Test: CSF drawing during spinal anaesthesia; Diagnostic Test: Fasting blood sample; Diagnostic Test: Lumbar puncture

• Registration Number: NCT03381482
• Lead Sponsor: University Hospital, Lille

Brief Summary

In Alzheimer's disease (AD), neurofibrillary degeneration (NFD) is characterized by the intraneuronal aggregation of Tau proteins. The pathology progresses through a hierarchical pathway that may be associated with the intercellular transmission of pathology as demonstrated in our rat models. This transmission implies that Tau is actively secreted and may participate to the first steps of Tau pathology spreading. It is demonstrated in cell lines and animal models (rodents and non-human primates) that Tau is secreted not only in free forms but also in extracellular vesicles. If Tau is found in biological fluids before neuronal death it may represent an early marker of the NFD and will also define therapeutically targets. In this context, the aim is now to transfer this knowledge in humans and to decipher the nature of Tau secreted in plasma and cerebrospinal fluids collected from healthy controls to AD patients, and to decipher if the presence of tau inside vesicles is influenced by the pathology.

Detailed Description

Not available

Study Timeline

• Study First Submitted: 2017-12-18
• Study First Submitted QC: 2017-12-18
• Study Start: 2017-12-20
• Study First Posted: 2017-12-22
• Status Verified: 2023-02
• Last Update Submitted: 2023-02-06
• Last Update Posted: 2023-02-08
• Primary Completion: 2023-12
• Study Completion: 2023-12

Recruitment & Eligibility

• Status: RECRUITING
• Sex: All
• Target Recruitment: 100

Inclusion Criteria

• Subjects able to undergo a lumbar puncture;
• Subjects who have a partner who will be required for driving back the subject after the lumbar punction for safety reasons (not required for control subjects);
• Subjects (or the study partner for group 5) capable of and willing to comply with the protocol and to give their written informed consents after having received and understood the subject information. According to the legal protection or the mental capacities of the subject, he/she will be accompanied by him/her legally acceptable representative during this procedure;
• Blood coagulation testing
• Subjects registered with the French Social Security, in agreement with the French law on biomedical experimentation.

Group 1: controls

• absence of cognitive complaint
• absence of significant cognitive impairment: MMSE>27
• Negative ApoE4 status (ε 4-/ ε 4-) No family history of AD at first degree Group 2: asymptomatic cases with high risk to develop AD
• absence of cognitive complaint
• absence of significant cognitive impairment : MMSE>27
• known ApoE4 status or family history of AD at first degree Group 3: cases with isolated cognitive complaint
• presence of a cognitive complaint
• absence of cognitive impairment assessed by MMSE>27 and standard neuropsychological examination (performed < 1 year) Group 4: prodromal AD according to the 2007 criteria (Dubois et al., 2007)
• progressive and significant episodic memory impairment >6 months
• And at least one of the following: medial temporal atrophy of brain MRI / low Ab42 and increased total and phosphorylated Tau protein in the CSF/ bilateral temporoparietal hypometabolism on brain FDG-PET/ positive amyloid brain PET if available
• exclusion of any differential diagnoses Group 5: Mild to moderate probable AD-type dementia according to the NIA 2011 criteria
• progressive and significant cognitive decline >6 months
• amnestic or any other predominant clinical presentation
• exclusion of any differential diagnoses
• MMSE between 15 and 26 (inclusive)

Exclusion Criteria

• Subjects with dementia caused by a non-neurodegenerative disease, including patients with severe cerebrovascular risk factor load;

Associated Illnesses or conditions:

• Subjects with other neurodegenerative disease such as fronto-temporal dementia (FTD), Lewy body dementia and Parkinson's disease;
• Subjects with other serious neurological disorder such as brain tumour, stroke, epilepsy, hydrocephalus and any condition which contraindicates, in the investigator's judgment, entry to the study;
• Subjects with demyelinating diseases of the peripheral nervous system such as Guillain-Barre Syndrome;

Biological exclusion criteria:

• Subjects with known active Hepatitis C Virus (HCV), Hepatitis B Virus (HBV) or Human Immunodeficiency Virus (HIV);
• Subjects with clinical or significant laboratory abnormalities, in the judgment of the investigator;

Others:

• Subjects with excessive alcohol intake or drug abuse, in the judgment of the investigator;
• Subjects who have contraindications to perform a lumbar puncture;
• Subjects who, in the opinion of the Investigator, have a risk of non-compliance to the study procedures or who are otherwise not appropriate to include in this clinical trial (for example, being impossible to contact in case of emergency).

Study & Design

• Study Type: OBSERVATIONAL
• Study Design: Not specified

Arm && Interventions

Group	Intervention	Description
Controls	CSF drawing during spinal anaesthesia	Group 1: the 4ml of CSF collected in the surgery context will be kept for the study, and 6x5ml of blood will be added to the usual samples.
Mild to moderate probable AD-type dementia	Lumbar puncture	Group 5: 10ml of CSF and 6x5ml of blood will be collected
Cases with isolated cognitive complaint	Fasting blood sample	Group 3: 10ml of CSF and 6x5ml of blood will be collected
Mild to moderate probable AD-type dementia	Fasting blood sample	Group 5: 10ml of CSF and 6x5ml of blood will be collected
Asymptomatic cases with high risk to develop AD	Lumbar puncture	Group 2: 10ml of CSF and 6x5ml of blood will be collected
Cases with isolated cognitive complaint	Lumbar puncture	Group 3: 10ml of CSF and 6x5ml of blood will be collected
Prodromal AD	Lumbar puncture	Group 4: 10ml of CSF and 6x5ml of blood will be collected
Controls	Fasting blood sample	Group 1: the 4ml of CSF collected in the surgery context will be kept for the study, and 6x5ml of blood will be added to the usual samples.
Asymptomatic cases with high risk to develop AD	Fasting blood sample	Group 2: 10ml of CSF and 6x5ml of blood will be collected
Prodromal AD	Fasting blood sample	Group 4: 10ml of CSF and 6x5ml of blood will be collected

Primary Outcome Measures

Name	Time	Method
Presence of Tau in extracellular vesicles in CSF	Baseline	Tau will be measured by ELISA in extracellular vesicles and the presence of Tau in extracellular vesicles will considered positive if the concentration of Tau is superior to the sensitivity threshold of the antibody used.

Secondary Outcome Measures

Name	Time	Method
The ratio of free Tau/vesicular Tau for all groups will be assessed with samples obtained during the visit.	Baseline	Tau will be measured by ELISA (concentration of Tau in pg/mL) and using the Nanosight technology (% of vesicles containing Tau). Results will be expressed either in percentage or in concentration (ie concentration of free Tau/concentration of vesicular Tau; % of free Tau/% of vesicular Tau).
The presence of clusters of the epigenetic markers H3K9me3 in nuclei of peripheral blood mononuclear cells for all groups will be assessed with samples obtained during the visit.	Baseline	The H3K9m3 marker will be revealed by immunodetection and revealed by fluorescence. The presence of one cluster of H3K9m3 will be considered as positive. Results will be expressed in % of cells with clusters.

Trial Locations

Locations (1)

Hôpital Roger Salengro, CHRU; 🇫🇷 Lille, France