Monika Hundelt scite author profile

Tau becomes characteristically altered both functionally and structurally in several neurodegenerative diseases now collectively called tauopathies. Although increasing evidence supports that alterations of tau may directly cause neuronal degeneration and cell death, the mechanisms, which render tau to become a toxic agent are still unclear. In addition, it is obscure, whether neurodegeneration in tauopathies occurs via a common mechanism or specific differences exist. The aim of this review is to provide an overview about the different experimental models that currently exist, how they are used to determine the role of tau during degeneration and what has been learnt from them concerning the mechanistic role of tau in the disease process. The review begins with a discussion about similarities and differences in tau alteration in paradigmatic tauopathies such as frontotemporal dementia and parkinsonism linked to chromosome 17 (FTDP-17) and Alzheimer's disease (AD). The second part concentrates on major experimental models that have been used to address the mechanistic role of tau during degeneration. This will include a discussion of cell-free assays, culture models using cell lines or dissociated neurons, and animal models. How these models aid to understand (i) alterations in the function of tau as a microtubule-associated protein (MAP), (ii) direct cytotoxicity of altered tau protein, and (iii) the potential role of tau aggregation in neurodegenerative processes will be the central theme of this part. The review ends with concluding remarks about a general mechanistic model of the role of tau alteration and neuronal degeneration in tauopathies and future perspectives.

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Oxygenic Photosystem II: The Mutation D1−D61N in Synechocystis sp. PCC 6803 Retards S-State Transitions without Affecting Electron Transfer from Y_Z to P₆₈₀⁺

Hundelt

Hays

Debus

et al. 1998

Biochemistry

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Photosynthetic oxygen evolution is powered by photosystem II (PSII), in particular by the oxidized chl a-aggregate P680+, and catalyzed by the oxygen-evolving complex (Mn4X-entity) as well as a tyrosine residue (YZ). The role of particular amino acids as cofactors of electron and proton transfer or as modulators of the activity is still ill-defined. The effects of single-site mutations at the donor side of PSII on the partial reactions of water oxidation have been primarily studied in whole cells. Because of better signal-to-noise in oxygen-evolving core preparations more detailed information on the electronic, protonic, and electrostatic events is expected from studies with such material. We investigated cells and oxygen-evolving core preparations from the wildtype of Synechocystis sp. PCC 6803 and point-mutants of D1-D61. In cells, oxygen-release was slowed drastically in D61A (8-fold) and D61N (10-fold) compared to WT, whereas it remained unchanged in D61E within the time resolution of the measurements. In core preparations, the S1 --> S2 and S2 --> S3 transitions were slowed approximately 2-fold in D61N compared to WT. However, the nanosecond components of electron transfer from YZ to P680+ were unchanged in the same mutant. We conclude that substitution of a neutral residue for D1-D61 selectively affects electron-transfer events on the donor side of YZ.

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Photosynthetic water oxidation in Synechocystis sp. PCC6803: mutations D1-E189K, R and Q are without influence on electron transfer at the donor side of photosystem II

Clausen¹,

Winkler²,

Hays³

et al. 2001

Biochimica et Biophysica Acta (BBA) - Bioenergetics

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The oxygen-evolving manganese cluster (OEC) of photosynthesis is oxidised by the photochemically generated primary oxidant (P(+*)(680)) of photosystem II via a tyrosine residue (Y(Z), Tyr161 on the D1 subunit of Synechocystis sp. PCC6803). The redox span between these components is rather small and probably tuned by protonic equilibria. The very efficient electron transfer from Y(Z) to P(+*)(680) in nanoseconds requires the intactness of a hydrogen bonded network involving Y(Z), D1-His190, and presumably D1-Glu189. We studied photosystem II core particles from photoautotrophic mutants where the residue D1-E189 was replaced by glutamine, arginine and lysine which were expected to electrostatically differ from the glutamate in the wild-type (WT). Surprisingly, the rates of electron transfer from Y(Z) to P(+*)(680) as well as from the OEC to Y(ox)(Z) were the same as in the WT. With the generally assumed proximity between D1-His190 (and thus D1-Glu189) and Y(Z), the lack of any influence on the electron transfer around Y(Z) straightforwardly implies a strongly hydrophobic environment forcing Glu (acid) and Lys, Arg (basic) at position D1-189 into electro-neutrality. As one alternative, D1-Glu189 could be located at such a large distance from the OEC, Y(Z) and P(+*)(680) that a charge on D1-189X does not influence the electron transfer. This seems less likely in the light of the drastic influence of its direct neighbour, D1-His190, on Y(Z) function. Another alternative is that D1-Glu189 is negatively charged, but is located in a cluster of acid/base groups that compensates for an alteration of charge at position 189, leaving the overall net charge unchanged in the Gln, Lys, and Arg mutants.

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Proton release from water oxidation by photosystem II: similar stoichiometries are stabilized in thylakoids and PSII core particles by glycerol

et al. 1997

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During the four-stepped catalytic cycle of water oxidation by photosystem II (PSII) molecular oxygen is released in only one of the four reaction steps whereas the release of four protons is distributed over all steps. In principle, the pattern of proton production could be taken as indicative of the partial reactions with bound water. In thylakoids the extent and rate of proton release varies as function of the redox transition and of the pH without concomitant variations of the redox pattern. The variation has allowed to discriminate between deprotonation events of peripheral amino acids (Bohr effects) as opposed to the chemical deprotonation of a particular redox cofactor, and of water. In contrast, in thylakoids grown under intermittent light, as well as in PSII core particles the pattern of proton release is flat and independent of the pH. This has been attributed to the lack in these materials of the chlorophyll a,d-binding (CAB) proteins. We now found that a thylakoid-like, oscillatory pattern of proton release was restored simply by the addition of glycerol which modifies the protein-protein interaction. Being a further proof for the electrostatic origin of the greater portion of proton release, this effect will serve as an important tool in further studies of water oxidation.

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Photosystem II of green plants. Oxidation and deprotonation of the same component (histidine?) on S1∗ ⇒ S2∗ in chloride-depleted centers as on S2 ⇒ S3 in controls

Haumann¹,

Drevenstedt²,

Hundelt³

et al. 1996

Biochimica et Biophysica Acta (BBA) - Bioenergetics

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Cofactor X of photosynthetic water oxidation: electron transfer, proton release, and electrogenic behaviour in chloride-depleted Photosystem II

Hundelt¹,

Haumann²,

Junge³

1997

Biochimica et Biophysica Acta (BBA) - Bioenergetics

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Altered phosphorylation but no neurodegeneration in a mouse model of tau hyperphosphorylation

Hundelt

Fath

Selle

et al. 2011

Neurobiology of Aging

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The Mutation D1-D61N in PS II of Synechocystis: Retardation of et from Oec→Y Z OX and No Effect on YZ→P 680 +

Hundelt

Hays

Debus

et al. 1998

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Monika Hundelt

Tau alteration and neuronal degeneration in tauopathies: mechanisms and models

Oxygenic Photosystem II: The Mutation D1−D61N in Synechocystis sp. PCC 6803 Retards S-State Transitions without Affecting Electron Transfer from Y_Z to P₆₈₀⁺

Photosynthetic water oxidation in Synechocystis sp. PCC6803: mutations D1-E189K, R and Q are without influence on electron transfer at the donor side of photosystem II

Proton release from water oxidation by photosystem II: similar stoichiometries are stabilized in thylakoids and PSII core particles by glycerol

Photosystem II of green plants. Oxidation and deprotonation of the same component (histidine?) on S1∗ ⇒ S2∗ in chloride-depleted centers as on S2 ⇒ S3 in controls

Cofactor X of photosynthetic water oxidation: electron transfer, proton release, and electrogenic behaviour in chloride-depleted Photosystem II

Altered phosphorylation but no neurodegeneration in a mouse model of tau hyperphosphorylation

The Mutation D1-D61N in PS II of Synechocystis: Retardation of et from Oec→Y Z OX and No Effect on YZ→P 680 +

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Monika Hundelt

Tau alteration and neuronal degeneration in tauopathies: mechanisms and models

Oxygenic Photosystem II: The Mutation D1−D61N in Synechocystis sp. PCC 6803 Retards S-State Transitions without Affecting Electron Transfer from YZ to P680+

Photosynthetic water oxidation in Synechocystis sp. PCC6803: mutations D1-E189K, R and Q are without influence on electron transfer at the donor side of photosystem II

Proton release from water oxidation by photosystem II: similar stoichiometries are stabilized in thylakoids and PSII core particles by glycerol

Photosystem II of green plants. Oxidation and deprotonation of the same component (histidine?) on S1∗ ⇒ S2∗ in chloride-depleted centers as on S2 ⇒ S3 in controls

Cofactor X of photosynthetic water oxidation: electron transfer, proton release, and electrogenic behaviour in chloride-depleted Photosystem II

Altered phosphorylation but no neurodegeneration in a mouse model of tau hyperphosphorylation

The Mutation D1-D61N in PS II of Synechocystis: Retardation of et from Oec→Y Z OX and No Effect on YZ→P 680 +

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Product

Resources

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Oxygenic Photosystem II: The Mutation D1−D61N in Synechocystis sp. PCC 6803 Retards S-State Transitions without Affecting Electron Transfer from Y_Z to P₆₈₀⁺