Summary

Neurodegeneration in an Animal Model of Chronic Amyloid-beta Oligomer Infusion Is Counteracted by Antibody Treatment Infused with Osmotic Pumps

Published: August 14, 2016
doi:

Summary

To study the effects of Aβo in vivo, we developed a model based on repeated hippocampal infusions of soluble Aβo coupled with continuous infusion of Aβo antibody (6E10) in the hippocampus using osmotic pumps to counteract the neurotoxic effect of Aβo.

Abstract

Decline in hippocampal-dependent explicit memory (memory for facts and events) is one of the earliest clinical symptom of Alzheimer's disease (AD). It is well established that synapse loss and ensuing neurodegeneration are the best predictors for memory impairments in AD. Latest studies have emphasized the neurotoxic role of soluble amyloid-beta oligomers (Aβo) that begin to accumulate in the human brain approximately 10 to 15 yr before the clinical symptoms become apparent. Many reports indicate that soluble Aβo correlate with memory deficits in AD models and humans. The Aβo-induced neurodegeneration observed in neuronal and brain slice cultures has been more challenging to reproduce in many animal models. The model of repeated Aβo infusions shown here overcome this issue and allow addressing two key domains for developing new disease modifying therapies: identify biological markers to diagnose early AD, and determine the molecular mechanisms underpinning Aβo-induced memory deficits at the onset of AD. Since soluble Aβo aggregate relatively fast into insoluble Aβ fibrils that correlate poorly with the clinical state of patients, soluble Aβo are prepared freshly and injected once per day during six days to produce marked cell death in the hippocampus. We used cannula specially design for simultaneous infusions of Aβo and continuous infusion of Aβo antibody (6E10) in the hippocampus using osmotic pumps. This innovative in vivo method can now be used in preclinical studies to validate the efficiency of new AD therapies that might prevent the deposition and neurotoxicity of Aβo in pre-dementia patients.

Introduction

It was initially proposed that accumulation of insoluble Aβ species in the brain was central to AD pathogenesis.1,2 However, amyloid plaques are also detected in some cognitively normal elderly.3-7 To overcome the poor correlation existing between plaque depositions and cognitive deficits in AD, latest reports have shown the presence of toxic soluble Aβo at the onset of the disease, which correlate much better with the clinical state of the patients.8-14 Since the process of Aβ oligomerization is very dynamic, it was suggested that neurotoxicity is induced by various Aβo instead of only one specific type of oligomer.14-16 Since many studies have shown that Aβo can initiate synapse dysfunctions prior to synapse and neuronal loss,17-24 current theories indicate that Aβ-related treatment might be effective in early AD rather than at later stages as tested so far in clinical trials.

One hallmark feature of AD pathogenesis is the massive and widespread cell death observed in the late stages of the disease, and the significant synapse and neuronal loss observed in localized brain regions when memory deficits become detectable at the clinical level. The perforant pathway that projects from the entorhinal cortex (EC) to the dentate gyrus (DG) is perturbed markedly at the early onset of AD.25,26 During the prodromal state of AD when mild cognitive impairment (MCI) becomes apparent significant cell death is detected in the EC as well as synaptic loss in the DG.25,26

Although a large body of evidence has pinpointed the toxic action of soluble Aβo in early AD,8-14 Aβo-induced neurodegeneration observed in neuronal culture or organotypic brain slice culture has been more challenging to reproduce in animal models.27 Most of the transgenic AD models overexpressing Aβ have amyloid plaques, tau hyperphosphorylation, synaptic deficiency and memory deficits.27 However, these models have been much less successful in modelling cell death observed in the hippocampus of AD patients. To overcome these technical issues we developed a model based on intracerebral infusions of soluble Aβo. We reported earlier that repeated hippocampal infusions of soluble Aβo induce gradual neuronal loss and tau hyperphosphorylation, two pathological hallmarks associated with memory decline in AD.28 Here, we are showing a novel method to test AD therapies using cannula specially design for simultaneous infusions of Aβo and continuous infusion of Aβo antibody (6E10) with osmotic pumps.

Osmotic pumps provide a unique way to test in vivo the efficiency of any antibody (or other compounds) against Aβo-induced neurodegeneration directly at the infusion site of Aβo. Thus, these pumps represent a convenient tool to establish a solid proof-of-concept regarding the mechanisms of action of potential therapeutic agents in AD. Since recent reports point out the critical impact of soluble Aβo in the early stages of AD, many treatments directed toward Aβo are actually being tested by academic and pharmaceutical laboratories. This novel animal model allows mimicking the synaptic and neuronal loss observed in early AD, and osmotic pumps are used to infuse continuously treatment agents specifically at the Aβo infusion site. The repetitive failures of AD therapies tested over the last few years in mild to moderate patients as prompted researchers to initiate trials in pre-dementia patients before Aβo begin to accumulate abundantly and generate irreversible brain damage. In this context, testing new compounds that prevent the deposition and consequently the neurotoxicity of Aβo might be of interest in pre-clinical patients.

Protocol

Ethics statement: The animal protocol for this project obtained the approval from the Animal Care Committee of the Hôpital du Sacré-Coeur de Montréal in compliance with the guidelines of the Canadian Council on Animal Care.

1. Catheter Preparation before Stereotaxic Surgery

  1. Cut PE50 catheters (6 cm in length) that will be used to connect cannula with osmotic pumps (see Figure 1A). Fill PE50 catheters with artificial cerebrospinal fluid (aCSF) and seal both ends of the catheters. Keep the catheter at 4 °C until used.

2. Cannula Implantation by Stereotaxy

  1. Perform the surgery in sterile conditions. Sterilize all the surgical instruments and materials by autoclaving. Clean the stereotaxic apparatus and the working area thoroughly, and disinfected with a 70% ethanol solution. Wear a surgical mask, hair bonnet and sterile gloves.
  2. Anesthetize rats by injecting intraperitoneally (i.p.) a solution of ketamine and xylazine (100 mg/kg and 10 mg/kg, respectively). Confirm anesthesia by checking movement after a gentle toe pinch.
  3. Inject a non-steroidal anti-inflammatory drug (Meloxicam; 1 mg/kg) subcutaneously (s.c.) to the anesthetized-animal at least 30 min prior to surgery.
  4. Shave the head of the animal using clippers and disinfect the skin with a solution of chlorhexidine gluconate 2% and isopropyl alcohol 2% three times. Apply veterinary ophthalmic ointment on eyes to prevent dryness while under anesthesia.
  5. Place the animal on a stereotaxic frame with the ear bars. Fix one cannula on the holder arm of the stereotaxic frame. Inject (s.c.) a local anesthetic agent (bupivacaine (1.5 mg/kg) and lidocaine (1.5 mg/kg) on the top of the head. Anesthesia is maintains during the whole procedure by placing a nose cone delivering 3% isoflurane. The entire surgical field should be draped off, but it was not done here to better demonstrate the technique.
  6. Make an incision of 3 cm on the top of the head with a scalpel. Install 4 clamps around the incision to leave the skull clear. Using a round-tip scissor, make a pocket (2 x 2 cm2) under the skin between shoulder blades of the animal.
  7. Scrape the periosteum of the skull with a blade. Apply a gauze pad on the skull if bleeding.
  8. Verify that the skull is flat and well aligned on the stereotaxic frame. To make sure that the skull is flat, check the height coordinates at the bregma and at the lambda. Take the coordinates of the bregma that will be used as the reference point.
  9. Starting from the bregma, calculate the coordinates of the two guide cannula that will be implanted bilaterally in the hippocampus (anteroposterior: – 0.42 cm; mediolateral: ± 0.30 cm; dorsoventral: – 0.28 cm according to the Paxinos and Watson rat brain atlas)29. Indicate the position of the cannula with a marker.
  10. Drill a hole (0.5 mm) in the skull at the implantation point of both cannula. Drill two other holes approximately 5 mm above and below those points to insert screws that will solidify cannula when applying dental cement.
  11. Cut one end of the catheter previously filled with aCSF with a scalpel, and insert it in the angle arm of the cannula. Fix the first cannula with dental cement. Avoid putting dental cement around the position on the second cannula.
  12. Let the dental cement dry for 2 – 3 min, then remove the holder arm from the first cannula, and fix the second cannula in it. Repeat steps 2.11 and 2.12. Put dummy cannula on both guide cannula. Ensure that the dummy and guide cannula are of the same length to prevent tissue infiltration and blocking the cannula.
  13. Insert the free end of both catheters in the pocket previously made between shoulder blades of the animal. Remove the clamps and stitch the skin with a suture thread 4-0.
    NOTE: The top guide cannula needs to be accessible for upcoming Aβo infusions.
  14. Remove the animal from the stereotaxic frame and put it back in its cage. During post-surgical recovery, place the cage on a heating water blanket until the animal wakes up. The cage should be partially on the pad so the rat can move away from the heat if needed.  Monitor the animal constantly until it regains sufficient consciousness to maintain sternal recumbency.
  15. Return rats to the animal facility to recover from the surgery for 10 days under close monitoring.
    NOTE: Do not return an animal that has undergone surgery to the company of other animals until fully recovered. Meloxicam (1 mg/kg) is given once per day during two days following surgery to treat pain.

3. Osmotic Pump Installation

  1. One day before installation, fill osmotic pumps with 6E10 antibody (1 mg/ml; 100 µl) and control IgG1 antibody (1 mg/ml; 100 µl) according to the manufacturer's instructions under sterile condition. Keep the pumps in sterile distilled water at 37 °C overnight to activate pumps.
  2. Anesthetize rats with isoflurane 3% to install osmotic pumps (0.5 µl/hr for 7 days). Shave between shoulder blades and disinfect the skin with a solution of chlorhexidine gluconate 2% and isopropyl alcohol 2%. Make an incision of 2 cm with a scalpel between shoulder blades to locate the PE50 catheters connected to the guide cannula.
  3. Cut the end of the PE50 catheters containing dental cement with a scalpel. Connect the osmotic pumps to the PE50 catheters, and add some dental cement at the pump and catheter junction to secure the connection.
  4. Stitch the skin tightly with a suture thread 4-0. Put the animal back in its cage on a heating water pad. Observe the animal wake up rapidly from an isoflurane anesthesia (about 5 min).
    NOTE: The surgery takes approximately 5 to 10 min.

4. Aβo Infusions in Awake and Freely Moving Rats

  1. Prepare the Aβo solution (0.2 µg/µl) as previously reported.28,30 Allow Aβo to aggregate dynamically and spontaneously for 1 hr at room temperature before infusion.
  2. Install two 10 µl syringes on an infusion pump. Fill the syringes with 5 µl of sterile distilled water. Cut two PE50 catheters to about 60 cm in length with a scalpel. Fill both catheters with sterile distilled water using 1 ml syringes and 21G needles.
  3. Keep the 1 ml syringes at one end of the catheter and connect the other end to the Hamilton syringes. Remove the 1 ml syringes and check that there is no air bubbles within the catheters.
  4. Insert internal cannula at the end of PE50 catheters. Using sterile distilled water, fill the internal cannula connected to PE50 catheters up to1 µl on Hamilton syringes. Make an air bubble by pulling back the pistons up to 2 µl.
  5. Mix the Aβo solution by pipetting up and down using a tip of minimum of adherence. Avoid forming bubbles during mixing. Fill both internal cannula with 1.5 µl of Aβo solution by pulling back the pistons up to 3.5 µl.
  6. Make lines with a marker before and after the air bubble done in both catheters. This serves as a check point of ongoing infusion. For infusion, bring the cage near the infusion pump and remove its cover.
  7. Place the rat in a snuggle and tightly scrape the arm of the snuggle around its neck to immobilize the head of the rat. Remove dummy cannula from the two guide cannula. Insert the internal cannula previously prepared in the guide cannula. Verify that they are fully inserted and well-fixed to the base of the guide cannula.
  8. Release rat from the snuggle and put it back in its cage to limit contention stress. Monitor closely to ensure that the catheters do not twist together and the infusion is done properly.
  9. Turn on the infusion pump. Inject 1 µl of Aβo solution at a rate of 0.1 µl/min (10 min). During infusion, check that the syringe piston moves from 3.5 µl to 2.5 µl, and that the air bubble in both PE50 catheters move continuously.
  10. Leave the internal cannula in place for another 5 min after infusion to allow efficient diffusion of Aβo solution. Bring the rat back in the snuggle to remove internal cannula and capped guide cannula to prevent reflux of the injected solution. Use dummy cannula that stop just before the angle arm of the cannula. Return the animal in its cage.
  11. Repeat Aβo infusion once per day over 6 consecutive days. Euthanize the animal by decapitation.

Representative Results

The neurotoxic effect of Aβo was investigated in Long-Evans rats by implanting cannula in the DG of the hippocampus. Soluble Aβo were injected every day over six consecutive days. We used cannula specially design for simultaneous infusions of Aβo and continuous infusion of 6E10 or control IgG1 antibody in the hippocampus using osmotic pumps (Figure 1A). For immunohistochemistry rats were anesthetized, perfused transcardially with 0.9% NaCl, and brains immersed in 4% paraformaldehyde solution for 48 hr and 15% sucrose solution for 24 hr. Free-floating coronal sections (40 µm) were treated with 0.3% H2O2 for 30 min, blocked in 1% goat serum for 1 hr, and incubated overnight at 4 °C with an anti-pan-Aβ antibody. Sections were treated with 70% formic acid for 3 min before applying the antibody. Detection was performed using the ABC complex and a 0.05% 3,3-diaminobenzidine solution. Sections were mounted on gelatin-coated glass slides, air-dried 2 hr, dehydrated (30, 70, 95, and 100% alcohol), incubated in toluene 5 min, and coverslipped. For cresyl violet staining, sections were incubated 10 min in a 0.5% cresyl violet solution, incubated 1 min in a 0.5% acetic acid solution, decolored (70, 95, and 100% alcohol), immersed in toluene 5 min, and covered with glass coverslip.

The results presented here show the deposition of Aβo in the DG in vicinity of the infusion site, and cell death associated with this accumulation. We found that the level Aβo was substantially decreased by 6E10 antibody treatment (Figure 1B). Marked neurodegeneration was observed near the injecting site of Aβo, and was attenuated by 6E10 antibody treatment (Figure 1B). These results are consistent with Aβo accumulation that we observed in the DG following repeated Aβo infusions in mice.28 Clearance of amyloid deposition by immunotherapy with 6E10 antibody shown here is in line with another report done in a transgenic AD mouse model.31

Figure 1
Figure 1. Photo of the Animal with Bilateral Cannula During Aβo Infusion. A solution of Aβo (0.2 µg/µl; 1 µl) was injected in awake and freely moving rats (once a day for 6 days) using PE50 catheters connected to internal cannula inserted into guide cannula. Treatment with control (Ctl) IgG1 or 6E10 antibody was infused directly at the site of Aβo infusion using osmotic pumps located subcutaneously between the shoulder blades of the animal. Please click here to view a larger version of this figure.

Figure 2
Figure 2. Neuronal Loss Induced by Aβo Deposition is Attenuated by 6E10 Antibody Treatment. A, Aβo (0.2 µg/µl; 1 µl) was injected once a day during 6 consecutive days, and treated with Ctl (IgG1) or 6E10 antibody at the site of infusion using osmotic pumps. B, Representative accumulation of Aβo in the DG on a section immediately next to cannula insertion, and representative staining with cresyl violet showing cell loss. Scale bars: 50 µm (n = 4) Please click here to view a larger version of this figure.

Discussion

There are critical steps within this protocol that required special attention. When implanting the cannula, avoid putting dental cement when it is too liquid to prevent blocking the hole of the second cannula. It is important to place dental cement at the free end of the P50 catheter attached to the pump to prevent irritation and a possible inflammatory response. The day of the stereotaxic surgery, use dummy cannula that are the same length as guide cannula to avoid blocking cannula. However, after installing pumps use shorter dummy cannula that stop before the angle arm of the cannula to allow proper infusion of the solution from the pump to the hippocampus. Monitor closely Aβo infusions and verify that the air bubble done in catheters is moving continuously during infusions. Always make sure that the injecting cannula is completely inserted into the guide cannula during infusions.

If problem is encounter during Aβ infusion, verify that the internal cannula is not blocked. If it is the case, flush sterile distilled water through the internal cannula. If the guide cannula is obstructed, turn the internal cannula into the guide cannula. Otherwise move the internal cannula up and down. Contention in the snuggle can be stressful for rats, especially on the first day. To decrease the stress of the animal, we recommend to manipulate and habituate rats to the snuggle before the stereotaxic surgery.

Many advantages can be attributed to this novel and flexible in vivo approach. Indeed, the nature of Aβo injected can be accurately control before infusion, and different type of Aβ preparations (for example synthetic vs brain-derived Aβ solutions) can be injected to evaluate their neurotoxicity in vivo. This model can also be used to investigate mechanisms by which various Aβ species (e.g., monomers, low- and high-molecular-weight oligomers, protofibrils) can induce neurotoxic effects in vivo, and how treatments like immunotherapy might counteract their deleterious impact in the brain. Since the infusions are perform in awake, freely-moving animals, there are no confounding effects between anesthetic agents and the Aβo solution on signaling pathways, as shown in previous studies.32,33 Infusions in freely moving animal are also compatible with behavioral testing any time before and after the infusions.

Infusions of Aβo and pump installation can be done in animal of different ages to determine the effects of Aβo and treatments during aging. Since neurodegeneration occurs in vicinity of the infusion site, synapse and neuronal loss can be induced in different and localized brain regions. The collateral infusion of Aβo and control (vehicle or scramble Aβ) allows controlling for any change within the same animal. Conversely, Aβo or control solutions can be injected bilaterally in the right and left hippocampus, for example when testing animals in behavioral tasks. Infusion of Aβo and treatment can be done simultaneously or alternatively pumps can be installed after Aβo infusion to evaluate if the treatment is effective after Aβ deposition. The same protocol described here can also be used when doing intracerebroventricular infusions of Aβo. The effect of Aβo on intracellular signaling pathways can be evaluated before and after neuronal loss within a reasonably short time frame. The dose and number of Aβ infusions can also be adjusted to obtain a more or less severe Aβ pathogenicity.

Although very versatile, this technique has some limitations. Cannula implantation produces a mechanical disruption of the tissue and neuroinflammation in the first few days following surgery. Thus, it is essential to wait at least one week after surgery before starting Aβo infusion, and to add proper controls (injection of vehicle or inactive scramble Aβ) to take into account these events. Also, only a small volume of Aβo can be infused to limit diffusion of the solution.

The osmotic pumps represent a convenient and unique delivery method for preclinical validation of agents designed to prevent Aβ-induced neurodegeneration. Since immunotherapy with the 6E10 antibody has been shown previously to decrease Aβ accumulation in the brain,31 we used the 6E10 antibody as a proof-of-concept to validate our new in vivo approach. The used of osmotic pumps in this model might now be used to develop novel disease modifying therapies that could prevent the deposition and neurotoxicity of Aβo in pre-clinical AD patients.

Divulgazioni

The authors have nothing to disclose.

Acknowledgements

We thank Caroline Bouchard from the animal facility for the rat work. A.S. holds a J.A. De Sève master fellowship, and B.P. a COPSE fellowship from the Université de Montréal This work was funded by grants attributed to J.B. from FRQS-Pfizer and start-up funds from Hôpital du Sacré-Coeur de Montréal Research Center.

Materials

Artificial Cerebrospinal Fluid (aCSF) Harvard Apparatus 59-7316
PE50 Catheter thin wall Plastics one C232CT
Ketamine Hydrochloride (100 mg/mL) Bioniche 1989529
Xylaxine Hydrochloride (100 mg/mL) Bimeda 8XYL004C
Meloxicam (5 mg/mL) Norbrook 215670I01
Solution of chlorhexidine gluconate 2% and isopropyl alcohol 2% Carefusion 260100C
Lidocaine Hydrochloride Alveda Pharma 0122AG01
Bupivacaine Hydrochloride Hospira 1559
ophthalmic ointment Baussh and Lomb inc. 2125706
stereotaxic frame Stoelting 51600
stereotaxic cannula holder arm Harvard Apparatus 72-4837
Drill Dremel 8050-N/18
Guide Cannula Plastics one 326OPG/spc
Injection Cannula Plastics one C315I/spc
Dummy Cannula Plastics one C315DC/spc
Suture thread coated vicryl rapide 4-0 Ethicon VR2297
Dental Acrylic Cement Harvard Apparatus 72-6906
Screws JI Morris Company P0090CE125
6E10 antibody (mouse IgG1 isotype)  BioLegend 803003
Mouse IgG1 isotype control antibody Abcam AB18447
Alzet osmotic pumps model 1007D Durect corporation 290
Isoflurane Baxter CA2L9100
Amyloid-beta 1-42  rPeptide A-1163-1
Hamilton syringe (10 µL) Fisher Scientique 14815279
Infusion Syringe Pump CMA 402 Harvard Apparatus CMA8003110
Syringe 1 mL BD 309659
Needle 21G Terumo NN-2125R
Snuggle Lomir Biomedical RTS04

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Citazione di questo articolo
Sajadi, A., Provost, C., Pham, B., Brouillette, J. Neurodegeneration in an Animal Model of Chronic Amyloid-beta Oligomer Infusion Is Counteracted by Antibody Treatment Infused with Osmotic Pumps. J. Vis. Exp. (114), e54215, doi:10.3791/54215 (2016).

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