Although the genetic association of ApoE and Alzheimer disease has been known for more than 10 years now, and ApoE4 is indeed the only proven independent risk factor, these recent studies, including the papers in JBC (5,12) are helping to explain why ApoE is essential and how it works to prevent or facilitate Aβ aggregation, amyloid deposition, and clearance. More importantly, the fact that ABCA1 controls ApoE lipidation status and thus its proper function in the brain opens completely new directions for drug design and therapeutic interventions in Alzheimer disease (7). In this respect, it appears that the availability of brain cholesterol and phospholipids to different carriers is critical for their function, and maintaining the appropriate distribution of brain lipids rather than inhibition of their synthesis may have a protective or even therapeutic effect in AD.

References:
1. Grainger DJ, Reckless J, McKilligin E. Apolipoprotein E modulates clearance of apoptotic bodies in vitro and in vivo, resulting in a systemic proinflammatory state in apolipoprotein E-deficient mice. J.Immunol. 2004;173:6366-75. Abstract

2. Hamon Y, Broccardo C, Chambenoit O, Luciani MF, Toti F, Chaslin S, Freyssinet JM, Devaux PF, McNeish J, Marguet D, Chimini G. ABC1 promotes engulfment of apoptotic cells and transbilayer redistribution of phosphatidylserine. Nat Cell Biol. 2000 Jul;2(7):399-406. Abstract

3. Han X, Fagan AM, Cheng H, Morris JC, Xiong C, Holtzman DM. Cerebrospinal fluid sulfatide is decreased in subjects with incipient dementia. Ann Neurol. 2003 Jul;54(1):115-9. Erratum in: Ann Neurol. 2003 Nov;54(5):693. Abstract

4. Hirsch-Reinshagen V, Zhou S, Burgess BL, Bernier L, McIsaac SA, Chan JY, Tansley GH, Cohn JS, Hayden MR, Wellington CL. Deficiency of ABCA1 impairs apolipoprotein E metabolism in brain. J Biol Chem. 2004 Sep 24;279(39):41197-207. Epub 2004 Jul 21. Abstract

5. Hirsch-Reinshagen V, Maia LF, Burgess BL, Blain JF, Naus KE, McIsaac SA, Parkinson PF, Chan JY, Tansley GH, Hayden MR, Poirier J, Van Nostrand W, Wellington CL. The absence of ABCA1 decreases soluble apoE levels but does not diminish amyloid deposition in two murine models of Alzheimer's disease. J Biol Chem. 2005 Oct 5; [Epub ahead of print] Abstract

6. Koistinaho M, Lin S, Wu X, Esterman M, Koger D, Hanson J, Higgs R, Liu F, Malkani S, Bales KR, Paul SM. Apolipoprotein E promotes astrocyte colocalization and degradation of deposited amyloid-beta peptides. Nat Med. 2004 Jul;10(7):719-26. Epub 2004 Jun 13. Abstract

7. Koldamova RP, Lefterov IM, Staufenbiel M, Wolfe D, Huang S, Glorioso JC, Walter M, Roth MG, Lazo JS. The liver X receptor ligand T0901317 decreases amyloid beta production in vitro and in a mouse model of Alzheimer's disease. J Biol Chem. 2005 Feb 11;280(6):4079-88. Epub 2004 Nov 22. Abstract

8. LaDu MJ, Pederson TM, Frail DE, Reardon CA, Getz GS, Falduto MT. Purification of apolipoprotein E attenuates isoform-specific binding to beta-amyloid. J Biol Chem. 1995 Apr 21;270(16):9039-42. Abstract

9. Shibata M, Yamada S, Kumar SR, Calero M, Bading J, Frangione B, Holtzman DM, Miller CA, Strickland DK, Ghiso J, Zlokovic BV. Clearance of Alzheimer's amyloid-ss(1-40) peptide from brain by LDL receptor-related protein-1 at the blood-brain barrier. J Clin Invest. 2000 Dec;106(12):1489-99. Abstract

10. van den Elzen P, Garg S, Leon L, Brigl M, Leadbetter EA, Gumperz JE, Dascher CC, Cheng TY, Sacks FM, Illarionov PA, Besra GS, Kent SC, Moody DB, Brenner MB. Apolipoprotein-mediated pathways of lipid antigen presentation. Nature. 2005 Oct 6;437(7060):906-10. Abstract

11. Wahrle SE, Jiang H, Parsadanian M, Legleiter J, Han X, Fryer JD, Kowalewski T, Holtzman DM. ABCA1 is required for normal central nervous system ApoE levels and for lipidation of astrocyte-secreted apoE. J Biol Chem. 2004 Sep 24;279(39):40987-93. Epub 2004 Jul 21. Abstract

12. Wahrle SE, Jiang H, Parsadanian M, Hartman RE, Bales KR, Paul SM, Holtzman DM. Deletion of Abca1 increases Abeta deposition in the PDAPP transgenic mouse model of Alzheimer's disease. J Biol Chem. 2005 Oct 5; [Epub ahead of print] Abstract

View all comments by Radosveta Koldamova
View all comments by Iliya Lefterov

1. Whereas we and Wahrle et al. (12) found a considerable increase in insoluble Aβ peptides in APP23 and PDAPP mice, Hirsch-Reinshagen et al. (5) reported no change in insoluble Aβ fraction in APP/PS1 or in TgSwDI/B transgenic mice. This discrepancy could be explained by the expression of APP transgenes producing Aβ species with different ability to aggregate or propensity for clearance. In APP/PS1 and Tg-SwDI/B mice, the expression of PS1 or Swedish, Dutch, and Iowa triple-mutant APP increases the proportion of more hydrophobic Aβ peptides (5), which are known to aggregate faster and undergo inefficient clearance compared to Aβ40 peptide.

2. While ABCA1 deficiency in APP23 and Tg-SwDI/B (5) caused an increase in amyloid plaques and a trend towards increase in PDAPP mice (12), Hirsch-Reinshagen et al. did not find a difference in amyloid deposition in APP/PS1 mice (5), which were examined at the more advanced age in terms of AD pathology. One explanation could be a role for ABCA1 in the initial period of aggregation and accumulation of amyloid.

The main conclusion from these three studies (Hirsch-Reinshagen et al., Koldamova et al., and Wahrle et al.) is that there is a negative correlation between amyloid load and the level of soluble, properly lipidated ApoE in the brain. Two contrasting roles for ApoE on amyloid deposition have been proposed: one promoting amyloid deposition and another mediating Aβ clearance. The first is supported by numerous in vivo data demonstrating that in transgenic APP mice with genetically disrupted endogenous mouse ApoE, fibrillar thioflavin S-positive Aβ deposits in brain parenchyma and vasculature are virtually missing. The second one is supported by in vitro and in vivo data demonstrating that ApoE has an important role in Aβ clearance across blood-brain barrier (BBB) and by astrocytes, a process mediated primarily via LDL receptors LRP1 and LRP2 (6,9). The three present JBC papers help to explain these seemingly contradictory effects of ApoE on amyloid aggregation and clearance by the differential roles of its lipid-rich and lipid-poor states. First, ApoE binding to various LDL receptors depends on its lipidation status: Lipid-poor ApoE is a weak ligand for LRP and LDL receptors, and this could explain the decreased Aβ clearance in ABCA1-/- mice. Insufficient and poorly lipidated ApoE in brain decreases Aβ clearance and degradation, and its retention in CNS will consequently increase amyloid deposition. Second, it was demonstrated that lipid-poor ApoE is more effective than lipid-rich ApoE in promoting Aβ aggregation (8). Previous work by Holtzman’s and Wellington’s groups demonstrated that ApoE in CSF of ABCA1-/- mice, as well as ApoE secreted in the conditioned media of ABCA1-/- astrocytes, is in a lipid-poor state (4,11). Moreover, it is obvious that, as in the periphery of ABCA1-/- mice or Tangier patients, poorly lipidated ApoA-I and ApoE proteins in the brain are unstable and are subjected to fast catabolism, explaining their decreased level.

References:
1. Grainger DJ, Reckless J, McKilligin E. Apolipoprotein E modulates clearance of apoptotic bodies in vitro and in vivo, resulting in a systemic proinflammatory state in apolipoprotein E-deficient mice. J.Immunol. 2004;173:6366-75. Abstract

2. Hamon Y, Broccardo C, Chambenoit O, Luciani MF, Toti F, Chaslin S, Freyssinet JM, Devaux PF, McNeish J, Marguet D, Chimini G. ABC1 promotes engulfment of apoptotic cells and transbilayer redistribution of phosphatidylserine. Nat Cell Biol. 2000 Jul;2(7):399-406. Abstract

3. Han X, Fagan AM, Cheng H, Morris JC, Xiong C, Holtzman DM. Cerebrospinal fluid sulfatide is decreased in subjects with incipient dementia. Ann Neurol. 2003 Jul;54(1):115-9. Erratum in: Ann Neurol. 2003 Nov;54(5):693. Abstract

4. Hirsch-Reinshagen V, Zhou S, Burgess BL, Bernier L, McIsaac SA, Chan JY, Tansley GH, Cohn JS, Hayden MR, Wellington CL. Deficiency of ABCA1 impairs apolipoprotein E metabolism in brain. J Biol Chem. 2004 Sep 24;279(39):41197-207. Epub 2004 Jul 21. Abstract

5. Hirsch-Reinshagen V, Maia LF, Burgess BL, Blain JF, Naus KE, McIsaac SA, Parkinson PF, Chan JY, Tansley GH, Hayden MR, Poirier J, Van Nostrand W, Wellington CL. The absence of ABCA1 decreases soluble apoE levels but does not diminish amyloid deposition in two murine models of Alzheimer's disease. J Biol Chem. 2005 Oct 5; [Epub ahead of print] Abstract

6. Koistinaho M, Lin S, Wu X, Esterman M, Koger D, Hanson J, Higgs R, Liu F, Malkani S, Bales KR, Paul SM. Apolipoprotein E promotes astrocyte colocalization and degradation of deposited amyloid-beta peptides. Nat Med. 2004 Jul;10(7):719-26. Epub 2004 Jun 13. Abstract

7. Koldamova RP, Lefterov IM, Staufenbiel M, Wolfe D, Huang S, Glorioso JC, Walter M, Roth MG, Lazo JS. The liver X receptor ligand T0901317 decreases amyloid beta production in vitro and in a mouse model of Alzheimer's disease. J Biol Chem. 2005 Feb 11;280(6):4079-88. Epub 2004 Nov 22. Abstract

8. LaDu MJ, Pederson TM, Frail DE, Reardon CA, Getz GS, Falduto MT. Purification of apolipoprotein E attenuates isoform-specific binding to beta-amyloid. J Biol Chem. 1995 Apr 21;270(16):9039-42. Abstract

9. Shibata M, Yamada S, Kumar SR, Calero M, Bading J, Frangione B, Holtzman DM, Miller CA, Strickland DK, Ghiso J, Zlokovic BV. Clearance of Alzheimer's amyloid-ss(1-40) peptide from brain by LDL receptor-related protein-1 at the blood-brain barrier. J Clin Invest. 2000 Dec;106(12):1489-99. Abstract

10. van den Elzen P, Garg S, Leon L, Brigl M, Leadbetter EA, Gumperz JE, Dascher CC, Cheng TY, Sacks FM, Illarionov PA, Besra GS, Kent SC, Moody DB, Brenner MB. Apolipoprotein-mediated pathways of lipid antigen presentation. Nature. 2005 Oct 6;437(7060):906-10. Abstract

11. Wahrle SE, Jiang H, Parsadanian M, Legleiter J, Han X, Fryer JD, Kowalewski T, Holtzman DM. ABCA1 is required for normal central nervous system ApoE levels and for lipidation of astrocyte-secreted apoE. J Biol Chem. 2004 Sep 24;279(39):40987-93. Epub 2004 Jul 21. Abstract

12. Wahrle SE, Jiang H, Parsadanian M, Hartman RE, Bales KR, Paul SM, Holtzman DM. Deletion of Abca1 increases Abeta deposition in the PDAPP transgenic mouse model of Alzheimer's disease. J Biol Chem. 2005 Oct 5; [Epub ahead of print] Abstract

View all comments by Radosveta Koldamova
View all comments by Iliya Lefterov

The Holtzman laboratory found that PDAPP (APPV717F) mice crossed onto an ABCA1-/- background have significantly more Aβ deposited in their brains and have a higher prevalence of cerebral amyloid angiopathy (CAA). There were no differences in APP processing in young PDAPP, ABCA1-/- mice that would account for the higher level of Aβ deposition. Additionally, the PDAPP, ABCA1-/- mice accumulated insoluble ApoE in plaques at a higher rate than PDAPP, ABCA1+/+ mice, suggesting that lipid-poor ApoE is not only more amyloidogenic but also that it binds to fibrillar Aβ. Using the APP23 (APPK670N, M671L) mouse model, the Lefterov group also showed that deletion of ABCA1 resulted in increased deposition of total and fibrillar (thioflavine S-positive) Aβ, which was not a result of altered APP processing. The Lefterov laboratory found significantly higher amounts of CAA and associated microhemorrhage in APP23, ABCA1-/- mice than APP23, ABCA1+/+ mice. The Wellington laboratory bred ABCA1-/- mice to two other mouse models: Tg-SwDI/B (APPK670N, M671L, E693Q, D694N) and APP/PS1 (APPK670N, M671L, PS1 DeltaE9). They did not see significant changes in soluble or insoluble Aβ in brain. However, this lack of an effect on Aβ deposition is still interesting given that the large decreases in ApoE levels in ABCA1-/- mice were expected to lead to large decreases in Aβ deposition. The Wellington group also noted increased insoluble ApoE in the ABCA1-/-, TgSwDI/B and ABCA1-/-, APP/PS1 mice compared to their respective ABCA1+/+ controls once plaques developed, again suggesting that the lipid-poor state of ApoE in ABCA1-/- mice may increase the fibrillogenesis of Aβ. Overall, the findings these papers suggest that modifying the lipidation state of ApoE in the brain may influence AD pathogenesis and be a potential treatment target.

View all comments by David Holtzman
View all comments by Suzanne Wahrle

All three groups reported that ABCA1 deficiency led to an 80 percent reduction in soluble ApoE levels, independent of mouse strain or AD model. Impaired ApoE secretion from both primary astrocytes and microglia has been shown to occur in ABCA1-deficient cells (4) and might partially explain this phenomenon. Additionally, increased catabolism of the poorly lipidated ApoE...  Read more

All three groups reported that ABCA1 deficiency led to an 80 percent reduction in soluble ApoE levels, independent of mouse strain or AD model. Impaired ApoE secretion from both primary astrocytes and microglia has been shown to occur in ABCA1-deficient cells (4) and might partially explain this phenomenon. Additionally, increased catabolism of the poorly lipidated ApoE particles present in ABCA1-deficient brains is likely to occur, as has been demonstrated for peripheral ApoA1 in Tangier disease (5). Given that ABCA1 is required to maintain normal brain ApoE levels, and because ApoE plays a key role in AD pathogenesis, further studies elucidating the exact mechanisms by which ABCA1 participates in brain ApoE metabolism are warranted.

The other common result to all papers is that despite a large decrease in soluble ApoE levels, no reduction in amyloid burden was observed in any of the four AD models tested. This suggests that ApoE lipidation status, which is reduced in ABCA1-deficient animals, is a crucial regulator of amyloid formation. In addition, different Aβ species and their specific deposition pattern did not influence the amyloidogenic effect of lipid-poor ApoE. ABCA1-deficient mice on either Tg-SwD/I, PDAPP, or APP23 background had increased amyloid burdens compared to their wild-type controls, suggesting that neither their specific Aβ species nor its deposition pattern (predominantly vascular in the Tg-SwD/I and parenchymal in the PDAPP and APP23 models) modulates amyloid formation in the presence of poorly lipidated ApoE. Together, all three papers demonstrate that low levels of poorly lipidated ApoE support at least as much amyloid deposition as wild-type levels of normally lipidated ApoE. How lipidation of ApoE contributes to the process of Aβ fibrillization, deposition, and clearance remains to be fully elucidated.

Although the most important findings were indeed corroborated by all groups, some differences were present and may be primarily related to methodological variables and time of analysis. Firstly, Koldamova et al. report an increase in amyloid and Aβ burden in APP23 mice that lacked ABCA1. Wahrle et al. reported a significant increase in guanidine-extractable Aβ load, but did not detect a significant change in amyloid burden. Hirsch-Reinshagen et al. report an increase in amyloid load in the Tg-SwD/I model but no detectable change in amyloid load in APP/PS1 mice that lacked ABCA1, and no change in guanidine-extractable Aβ levels in either model. Even though all groups saw no reduction in amyloid deposition despite a large decrease in ApoE levels, the differences in amyloid and Aβ load between wild-type and ABCA1-deficient mice may have been dependent on the stage of progression of AD. For example, in the APP/PS1 model, where severe pathology was present at the moment of analysis, no differences were observed in amyloid burden or guanidine-extractable Aβ levels between wild-type and ABCA1-deficient mice. In all other three models, analyzed at relatively earlier stages of disease progression, ABCA1-deficient animals did show an increase in amyloid burden when compared to wild-type controls. Further studies might clarify whether the role of ApoE in amyloid formation is most important during the initial stages of Aβ fibrillization, or whether other differences among the models tested may account for the differences in Aβ compared to amyloid burden.

A second important difference among the three studies relates to the report of a shift in ApoE distribution from a soluble to an insoluble pool. Wahrle et al. and Hirsch-Reisnhagen et al. showed an increase in guanidine-extractable pool of ApoE in ABCA1-deficient brains compared to controls. Koldamova et al., using formic acid extractions, did not observe such a phenomenon. Again, it is unclear whether this discrepancy is only of methodological nature or if singularities of the mouse model used by Koldamova et al. are responsible for this. The mechanisms underlying the shift of ApoE into an insoluble form are probably closely related to the increased amyloidogenicity of lipid-poor ApoE and are therefore an interesting subject for further studies.

References:
1. Hirsch-Reinshagen V, Maia LF, Burgess BL, Blain JF, Naus KE, McIsaac SA, Parkinson PF, Chan JY, Tansley GH, Hayden MR, Poirier J, Van Nostrand W, Wellington CL. The absence of ABCA1 decreases soluble apoE levels but does not diminish amyloid deposition in two murine models of Alzheimer's disease. J Biol Chem. 2005 Oct 5; [Epub ahead of print] Abstract

2. Koldamova R, Staufenbiel M, Lefterov I. Lack of ABCA1 considerably decreases brain Apoe level and increases amyloid deposition in APP23 mice. J Biol Chem. 2005 Oct 5; [Epub ahead of print] Abstract

3. Wahrle SE, Jiang H, Parsadanian M, Hartman RE, Bales KR, Paul SM, Holtzman DM. Deletion of Abca1 increases Aβ deposition in the PDAPP transgenic mouse model of Alzheimer's disease. J Biol Chem. 2005 Oct 5; [Epub ahead of print] Abstract

4. Hirsch-Reinshagen V, Zhou S, Burgess BL, Bernier L, McIsaac SA, Chan JY, Tansley GH, Cohn JS, Hayden MR, Wellington CL. Deficiency of ABCA1 impairs apolipoprotein E metabolism in brain. J Biol Chem. 2004 Sep 24;279(39):41197-207. Epub 2004 Jul 21. Abstract

5. Oram JF. Tangier disease and ABCA1. Biochim Biophys Acta. 2000 Dec 15;1529(1-3):321-30. Review. Abstract

View all comments by Veronica Hirsch-Reinshagen
View all comments by Cheryl Wellington

The second paper by Lewis et al. took the opposite approach of breeding APP/PS1 mice with transgenic mice expressing human ApoA-I. There, studies found the opposite result where the triple transgenic mice had improved behavioral performance and decreased levels of CAA. Furthermore, this study went on to show that in the presence of ApoA-I there was a decrease in glial activation and pro-inflammatory cytokine production. Together, these studies further suggest that in addition to...  Read more

The second paper by Lewis et al. took the opposite approach of breeding APP/PS1 mice with transgenic mice expressing human ApoA-I. There, studies found the opposite result where the triple transgenic mice had improved behavioral performance and decreased levels of CAA. Furthermore, this study went on to show that in the presence of ApoA-I there was a decrease in glial activation and pro-inflammatory cytokine production. Together, these studies further suggest that in addition to its well-known cardiovascular effects, ApoA-I may also have profound effects in the CNS that may be important in the pathogenesis of AD.

On another point, I was particularly intrigued with how these two papers further support the concept studied in my lab, i.e. the relationship between CAA, neuroinflammation, and cognitive impairment. Earlier, we reported that cerebral microvascular amyloid deposition promotes neuroinflammation and behavioral deficits in the vasculotropic mutant APP mouse model Tg-SwDI (1,2). Reducing microvascular CAA in Tg-SwDI diminished the associated neuroinflammation, and this occurred in the absence of any changes in total Aβ load or the levels of soluble Aß oligomers (3).

This earlier finding is consistent with the present results of Lefterov et al. that show in the absence of ApoA-I worsening behavioral performance in the APP/PS1 mice was associated with increased CAA load, not the level of soluble Aβ oligomers. Moreover, specifically reducing CAA-induced microglial activation improved behavioral performance in Tg-SwDI mice further strengthening the link between CAA, neuroinflammation, and cognitive impairment (4).

These two papers indicate that ApoA-I fits as a protein that may be more specifically tailored towards the cerebral vascular contribution of AD and related disorders. First, Lefterov et al. show that ApoA-I hinders Aβ assembly into larger oligomeric/fibrillar structures and blocks their toxicity towards cultured human brain vascular smooth muscle cells. Proper assembly of Aβ is required for brain vascular smooth muscle cell toxicity (5,6). Second, ApoA-I may be intimately involved with efficient efflux of Aβ out of brain across the cerebral vasculature. Therefore, as the present two papers suggest, increasing or decreasing the expression of ApoA-I may have profound effects on the ability to clear Aβ at the level of cerebral blood vessel influencing the development of CAA. It would be interesting to determine what the plasma levels of Aβ are in these models with altered ApoA-I expression.

Finally, the anti-inflammatory properties of ApoA-I may directly suppress localized CAA-induced neuroinflammation. In any case, these two manuscripts support further investigation into the specific contribution of CAA to neuroinflammation and cognitive impairment and how endogenous molecules, such as ApoA-I, may influence these processes.

References:

1. Miao, J., Xu, F., Otte-Höller, I., Verbeek, M.M., Davis, J., and Van Nostrand, W.E. (2005) Cerebral microvascular Aβ deposition induces vascular degeneration and neuroinflammation in transgenic mice expressing human vasculotropic mutant AßPP. American Journal of Pathology 167:505-515. Abstract

2. Xu, F., Grande, A.M., Robinson, J.K., Previti, M.L., Davis, J., and Van Nostrand, W.E. (2007) Early-onset subicular microvascular amyloid and neuroinflammation correlate with behavioral deficits in vasculotropic mutant AβPP transgenic mice. Neuroscience 146:98-107. Abstract

3. Miao, J., Vitek, M.P., Xu, F., Previti, M.L., Davis, J., and Van Nostrand, W.E. (2005) Reducing cerebral microvascular amyloid β protein deposition diminishes regional neuroinflammation in vasculotropic mutant amyloid precursor protein transgenic mice. Journal of Neuroscience 25:6271-6277. Abstract

4. Fan, R., Xu, F., Previti, M.L., Davis, J., Grande, A.M., Robinson, J.K., and Van Nostrand, W.E. (2007) Minocycline reduces microglial activation and improves behavioral deficits in a transgenic model of cerebral microvascular amyloid. Journal of Neuroscience 27:3057-3063. Abstract

5. Van Nostrand, W.E., Melchor, J., and Ruffini, L. (1998) Pathogenic cell surface amyloid β-protein fibril assembly in cultured human cerebrovascular smooth muscle cells. Journal of Neurochemistry 70:216-223. Abstract

6. Van Nostrand, W.E. and Melchor, J.P. (2001) Disruption of pathologic amyloid β-protein fibril assembly on the surface of cultured human cerebrovascular smooth muscle cells. Amyloid 8:20-27. Abstract

View all comments by William Van Nostrand

There is now substantial evidence that the accumulation of soluble and insoluble amyloid beta (Aβ) in the brain is a major factor in the etiology of AD. Preventing the accumulation of Aβ in the brain or facilitating its removal has become a major therapeutic goal for Alzheimer’s disease. Aβ-immunotherapy removes insoluble plaques of Aβ from the brain, but it appears that Aβ becomes entrapped in the perivascular drainage pathways by which a proportion of the Aβ is normally eliminated and results in increased severity of cerebral amyloid angiopathy (CAA). In addition, levels of soluble Aβ in the brain rise as a further indication that immunotherapy does not result in the complete elimination of Aβ from the brain. This has emphasized the importance of the perivascular drainage routes in the elimination of Aβ from the brain.

The major impact of the experimental work published by Iliya Lefterov et al. is that it represents a step towards elucidating the role of major risk factors such as hypercholesterolemia and apolipoproteins in impeding the elimination of Aβ from the AD...  Read more

There is now substantial evidence that the accumulation of soluble and insoluble amyloid beta (Aβ) in the brain is a major factor in the etiology of AD. Preventing the accumulation of Aβ in the brain or facilitating its removal has become a major therapeutic goal for Alzheimer’s disease. Aβ-immunotherapy removes insoluble plaques of Aβ from the brain, but it appears that Aβ becomes entrapped in the perivascular drainage pathways by which a proportion of the Aβ is normally eliminated and results in increased severity of cerebral amyloid angiopathy (CAA). In addition, levels of soluble Aβ in the brain rise as a further indication that immunotherapy does not result in the complete elimination of Aβ from the brain. This has emphasized the importance of the perivascular drainage routes in the elimination of Aβ from the brain.

The major impact of the experimental work published by Iliya Lefterov et al. is that it represents a step towards elucidating the role of major risk factors such as hypercholesterolemia and apolipoproteins in impeding the elimination of Aβ from the AD brain. Lipidated and non-lipidated ApoA-I inhibit the aggregation and toxicity of both Aβ 40 and 42. Deletion of the mouse ApoA-I gene significantly worsened cognitive performance in APP/PS1 transgenic mice, but did not change the total Aβ load. The important aspect is that arterial CAA was increased. The authors suggest that this may be due to the formation of Aβ fibrils in the vicinity of blood vessels and/or the effect that ApoA-I has on the smooth muscle cells. However, this does not explain the 5:1 ratio of Aβ40:42 observed in the APP/PS1ΔE9/ApoA-Iko mice. We suggest that ApoA-I may act as a chaperone, facilitating the transport of Aβ along the basement membranes of cerebral arteries. The absence of ApoA-I may result in a disruption to the normal dynamics of perivascular drainage, resulting in the accumulation of Aβ in the walls of arteries.

The paper authored by Terry Lewis et al. describes high levels of HDL accompanied by unaltered levels of Aβ load, improved cognitive function and reduced neuroinflammation in the brains of APP/PS1 transgenic mice crossed with ApoA-I human replacement gene mice, compared to transgenic APP/PS1 mice. Overexpression of ApoA-I led to a reduction in CAA, although we do have concerns about using a non-specific dye (Congo red) as a sole marker for the amyloid deposition associated with blood vessels. These results suggest that ApoA-I facilitates the elimination of Aβ along the basement membranes of cerebral capillaries and arteries, but the overproduction of mutant Aβ in the extracellular spaces of the brain parenchyma leads to the formation of plaques and a rise in soluble Aβ.

The roles that ApoA and ApoE may have in the dynamics of perivascular drainage and clearance of Aβ from the brain remain to be explored.

View all comments by Roxana O. Carare
View all comments by Cheryl Hawkes