. Folate deficiency induces in vitro and mouse brain region-specific downregulation of leucine carboxyl methyltransferase-1 and protein phosphatase 2A B(alpha) subunit expression that correlate with enhanced tau phosphorylation. J Neurosci. 2008 Nov 5;28(45):11477-87. PubMed.

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  1. Methylation and Tau
    The wealth of reports in the last decade confirming an association between homocysteine and Alzheimer disease hint that disturbed methylation might somehow relate to AD pathology (Smith, 2008; McCaddon and Hudson, 2007). A link between impaired methylation and neurofibrillary tangle formation was first proposed by Scott and Vafai in 2002 (Vafai and Stock, 2002). In support of this elegant hypothesis Obeid et al. found an association between phospho-tau and the ratio of the methyl donor S-adenosylmethionine (SAM) and its demethylated product S-adenosylhomocysteine (SAH) in the CSF of 182 patients with various neurological disorders (Obeid et al., 2007).

    SAH is a potent inhibitor of methyltransferase reactions, and last year Sontag et al. found that exposing neuroblastoma cells to SAH led to reduced methylation of PP2A (Sontag et al., 2007). Sontag’s group now show that folate deprivation downregulates PP2A carboxymethyltransferase expression in these cells, ultimately resulting in cell death. Protection is afforded by overexpressing either the methyltransferase or the Balpha regulatory subunit of PP2A, whereas knockdown of either protein accelerates the toxicity of folate deprivation. Reduced SAM and elevated SAH concentrations in folate deficient mice are also associated with enhanced tau phosphorylation in susceptible brain regions.

    Importantly, this work suggests an association between methylation status and one of the key pathological features of Alzheimer disease. Impaired methylation is likely to have other widespread effects in the nervous system. For example, alterations in the SAM/SAH ratio are also associated with PS1 and BACE upregulation and β amyloid deposition (Fuso et al., 2008). ”Tau-ists” and ”Bap-tists”’ should both be aware that the ”Meth-odists” may well be on to something!

    References:

    . B-vitamin deprivation induces hyperhomocysteinemia and brain S-adenosylhomocysteine, depletes brain S-adenosylmethionine, and enhances PS1 and BACE expression and amyloid-beta deposition in mice. Mol Cell Neurosci. 2008 Apr;37(4):731-46. PubMed.

    . Alzheimer's disease, oxidative stress and B-vitamin depletion. Future Neurol. 2007 Sep;2(5):537-47.

    . Folate and methylation status in relation to phosphorylated tau protein(181P) and beta-amyloid(1-42) in cerebrospinal fluid. Clin Chem. 2007 Jun;53(6):1129-36. PubMed.

    . The worldwide challenge of the dementias: a role for B vitamins and homocysteine?. Food Nutr Bull. 2008 Jun;29(2 Suppl):S143-72. PubMed.

    . Protein phosphatase 2A methyltransferase links homocysteine metabolism with tau and amyloid precursor protein regulation. J Neurosci. 2007 Mar 14;27(11):2751-9. PubMed.

    . Folate deficiency induces in vitro and mouse brain region-specific downregulation of leucine carboxyl methyltransferase-1 and protein phosphatase 2A B(alpha) subunit expression that correlate with enhanced tau phosphorylation. J Neurosci. 2008 Nov 5;28(45):11477-87. PubMed.

    . Protein phosphatase 2A methylation: a link between elevated plasma homocysteine and Alzheimer's Disease. FEBS Lett. 2002 May 8;518(1-3):1-4. PubMed.

    View all comments by Andrew McCaddon
  2. This is a well-designed and very exhaustive investigation of the effect of the administration of retinoic acid in a good murine model of Alzheimer disease. The beneficial effects of retinoic acid administration are plausible, consistent, and substantial. It is heartening to me to read this paper since previous publications by my colleagues and me (Lerer et al., 2008; Goodman et al., 2008; Goodman, 2006; Palha and Goodman, 2006; Goodman and Pardee, 2003) have suggested that increasing levels of retinoic acid in the brain might have therapeutic effects in late-onset Alzheimer disease through targeting of the retinol binding proteins, transthyretin, the retinoic acid receptors, or the retinoid receptor inhibitors (CYP26s). Administering retinoic acid analogs might also have benefit.

    To my knowledge there are no clinical trials in humans addressing the use of retinoids in Alzheimer disease. However, recently a preliminary drug trial has been published (Lerer et al., 2008) testing the effect of administering very low doses of the retinoid x receptor ligand, bexarotene—LGD1069 (Targretin)—to patients with chronic schizophrenia. The hippocampus and other brain regions affected in schizophrenia are similar to those implicated in Alzheimer disease. The drug was well tolerated, with the exception of an increase in serum cholesterol levels, and the trial demonstrated significant reduction of chronic symptoms. The unique insight of this trial was the extreme dilution of the retinoid analog. The usual clinical dosage of 300 mg/day was reduced to 75 mg/day, still achieving significant symptom reduction. Whether such a paradigm could prove successful in the treatment of Alzheimer disease remains to be demonstrated.

    See also:

    Goodman AB, McCaffery P, Palha JA, Simons, C, Pardee AB. Enhancement of brain retinoic acid levels, Chapt. 8 in H. John Smith, Claire Simons, & Robert D. E. Sewell, “Protein Misfolding in Neurodegenerative Diseases” p. 337-378, CRC Press Taylor & Francis Group New York 2008.

    References:

    . Bexarotene as add-on to antipsychotic treatment in schizophrenia patients: a pilot open-label trial. Clin Neuropharmacol. 2008 Jan-Feb;31(1):25-33. PubMed.

    . Retinoid receptors, transporters, and metabolizers as therapeutic targets in late onset Alzheimer disease. J Cell Physiol. 2006 Dec;209(3):598-603. PubMed.

    . Thyroid hormones and retinoids: a possible link between genes and environment in schizophrenia. Brain Res Rev. 2006 Jun;51(1):61-71. PubMed.

    . Evidence for defective retinoid transport and function in late onset Alzheimer's disease. Proc Natl Acad Sci U S A. 2003 Mar 4;100(5):2901-5. PubMed.

    View all comments by Ann B Goodman
  3. Tauopathies are a group of diseases characterized by accumulation of tau protein. Tau protein has a novel physiological function in the brain—stabilizing the neurons. Alterations in the amount or the structure of tau protein might destabilize the microtubules, thus causing changes in subcellular structures like the lysosomes (1) or the mitochondria (2). Tau can be structurally modified by phosphorylation, glycosylation, oxidation, and crosslinking. These pathological forms of tau tend to form self-aggregates and thus forming the neurofibrilary tangles (NFTs). NFTs are typical findings in all tauopathies containing paired PHF comprising hyperphosphorylated tau (3).

    Alzheimer disease (AD) is the best known tauopathy that is characterized by accumulation of NFTs in the brain. In an animal model of neurodegenerative diseases, mice developed progressive accumulation of NFTs, neuronal loss, and memory decline (4). Suppressing the transgenic tau caused improvement in memory function, and neuron numbers stabilized. Unexpectedly, NFTs continued to accumulate. The authors concluded that tau accumulation rather than NFTs can cause cognitive decline or neuronal death in this model of tauopathy (4). Although, these results can not be extrapolated to humans without further research, they might suggest that lowering tau protein can improve cognitive function in humans as well (4).

    A very tempting hypothesis that would have implications for prevention and treatment of tauopathies is that lowering the modified forms of tau protein might protect the brain. The degree of tau phosphorylation and the phosphorylated residues regulate binding of tau to microtubules, thus affecting its function. There is a state of balance between kinase-mediated phosphorylation and phosphatase-mediated dephosphorylation. Tau can be phosphorylated by several kinases (proline and non-proline directed; glycogen synthase kinase 3, Cdk5, MAP kinase, JNK, PKC, calmodulin kinase II). Protein phosphatase 2A (PP2A) is the most important phosphatase in the brain acting on most phosphorylated sites of tau. PP2A is composed of three subunits: A, B, and C. The subunit Bα is involved in substrate recognition and is considered the regulatory subunit. The binary enzyme AC must be methylated on Leu-309 to be able to join the B subunit and form the functional enzyme. The methylation is mediated by leucine carboxy methyltransferase-1 (LCMT-1), an S-adenosyl methionine (SAM) dependent enzyme.

    In the recently published study by Sontag et al., the authors conducted several elegant experiments aiming at testing the effect of folate deprivation on the expression of hyperphosphorylated tau protein, PP2A enzyme and the methyltransferase required for its activation (5). The authors found that folate deficiency caused disturbed methylation potential in brain tissues. Furthermore, enhanced tau phosphorylation and cell death were related to downregulation of LCMT-1 and subsequent loss of ABαC complex. Folate deficiency caused an enhanced expression of the non-methylated form of PP2A enzyme. This condition did not change the existing PP2A, suggesting that binding of the ABαC complex is stable against demethylation by PME-1. In a previous study by Sontag et al., the authors found that mice fed a high methionine/low folate diet had higher brain S-adenosylhomocysteine (SAH) and lower expression of LCMT-1 (also called PP2A methyl transferase, or PPMT), thus leading to severe decrease of the steady state of PP2A (6). Another recent study found that SH-SY5Y neuroblastoma cells grown in a folate-deficient medium showed a decrease in the phosphatase activity, and this effect was reversible by adding SAM to the folate-deficient medium (7). Another interesting mechanism explaining the effect of folate deficiency on phosphorylated tau protein is related to enhancing activity of one or more of the kinases responsible for tau phosphorylation in the brain (7). This effect on the kinases is thought to be related to activating NMDA channels and thereby Ca++-dependent kinase pathways by homocysteine (Hcy). Therefore, folate deficiency is causally related to accumulation of tau protein; this effect is at least partly mediated by disturbed methylation status.

    The study by Sontag et al. opens new perspectives for future research dealing with the pathophysiology of dementia or studies aiming at developing protective or therapeutic measures (5). Methyl group metabolism is regulated by micronutrients such as folate, vitamin B12, and vitamin B6. Several methyl donors in human diet have been identified, such as methionine and choline. The role of folate ingested with the diet is to convert Hcy into methionine in the presence of methyl cobalamin. Methionine is activated in the presence of ATP and further converted into SAM. SAM is a methyl donor that participates in numerous biological reactions including DNA methylation, and metabolism of neurotransmitters and phospholipids. Betaine, a product of the nutrient choline, is an alternative methyl donor in the conversion of Hcy into methionine via homocysteine betaine methyltransferase. However, this pathway has probably no or a limited role in Hcy remethylation in the brain. Furthermore, all factors that cause accumulation of Hcy (renal insufficiency, vitamin B deficiency, and alcoholism and liver disorders) might cause disturbed methylation potential. This metabolic condition implies increased S-adenosyl homocysteine (SAH) that acts as a potent inhibitor of methyltransferases by preventing SAM binding.

    Deficiency of micronutrients is common in elderly people. Among other environmental factors, both hyperhomocysteinemia and B-vitamin deficiencies have been linked to increased risk for dementia and other age-related neurodegenerative diseases. Therefore, enhancing B vitamin status has a great potential to prevent metabolic conditions, associated memory disorders, and dementia. Future studies should test in-vivo the role of micronutrients in preventing or reversing phospho-tau accumulation in the brain. It is equally important in such studies to control for all sources of methyl donors in the diet.

    References:

    . Lysosomes are associated with microtubules and not with intermediate filaments in cultured fibroblasts. Proc Natl Acad Sci U S A. 1984 Feb;81(3):788-92. PubMed.

    . KIF1B, a novel microtubule plus end-directed monomeric motor protein for transport of mitochondria. Cell. 1994 Dec 30;79(7):1209-20. PubMed.

    . Microtubule-associated protein tau. A component of Alzheimer paired helical filaments. J Biol Chem. 1986 May 5;261(13):6084-9. PubMed.

    . Tau suppression in a neurodegenerative mouse model improves memory function. Science. 2005 Jul 15;309(5733):476-81. PubMed.

    . Folate deficiency induces in vitro and mouse brain region-specific downregulation of leucine carboxyl methyltransferase-1 and protein phosphatase 2A B(alpha) subunit expression that correlate with enhanced tau phosphorylation. J Neurosci. 2008 Nov 5;28(45):11477-87. PubMed.

    . Protein phosphatase 2A methyltransferase links homocysteine metabolism with tau and amyloid precursor protein regulation. J Neurosci. 2007 Mar 14;27(11):2751-9. PubMed.

    . Folate deprivation increases tau phosphorylation by homocysteine-induced calcium influx and by inhibition of phosphatase activity: Alleviation by S-adenosyl methionine. Brain Res. 2008 Mar 14;1199:133-7. PubMed.

    View all comments by Wolfgang Herrmann

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