Your search keyword '"Neurofibrils ultrastructure"' showing total 544 results

1. Excitable neurofibrils and the problem of identifying the structure of central excitatory synapses in the nineteenth century.

Author

Bennett MR

Subjects

Action Potentials physiology, Animals, Dendrites physiology, Dendrites ultrastructure, Histology history, History, 19th Century, History, 20th Century, Humans, Neurofibrils physiology, Neurosciences history, Synapses physiology, Neurofibrils ultrastructure, Synapses ultrastructure

Abstract

Neurofibrils, identified after staining with Cajal's reduced silver nitrate, for example, were thought by many senior histologists in the nineteenth and early-twentieth centuries to conduct action potentials. There was no basis for this popular idea, although it was the impetus for intense study of the "neurofibrillar network" within neurons by Golgi, Cajal, Freud, and many others. Here, I trace the way in which this "excitable neurofibrillary" hypothesis led to major problems in the attempt by histologists to identify the central excitatory synapse, postulated by Sherrington on functional grounds and eventually described by Berkley.

Published

2015

2. Proteolytic cleavage of polymeric tau protein by caspase-3: implications for Alzheimer disease.

Author

Jarero-Basulto JJ, Luna-Muñoz J, Mena R, Kristofikova Z, Ripova D, Perry G, Binder LI, and Garcia-Sierra F

Subjects

Aged, 80 and over, Amino Acid Chloromethyl Ketones pharmacology, Aspartic Acid metabolism, Brain pathology, Brain ultrastructure, Caspase 3 metabolism, Female, Humans, Male, Microscopy, Electron, Molecular Weight, Neurofibrillary Tangles metabolism, Neurofibrillary Tangles pathology, Neurofibrillary Tangles ultrastructure, Neurofibrils metabolism, Neurofibrils pathology, Neurofibrils ultrastructure, Neuroprotective Agents pharmacology, Oligopeptides pharmacology, tau Proteins ultrastructure, Alzheimer Disease pathology, Brain metabolism, Caspase 3 pharmacology, tau Proteins drug effects, tau Proteins metabolism

Abstract

Truncated tau protein at Asp(421) is associated with neurofibrillary pathology in Alzheimer disease (AD); however, little is known about its presence in the form of nonfibrillary aggregates. Here, we report immunohistochemical staining of the Tau-C3 antibody, which recognizes Asp(421)-truncated tau, in a group of AD cases with different extents of cognitive impairment. In the hippocampus, we found distinct nonfibrillary aggregates of Asp(421)-truncated tau. Unlike Asp(421)-composed neurofibrillary tangles, however, these nonfibrillary pathologies did not increase significantly with respect to the Braak staging and, therefore, make no significant contribution to cognitive impairment. On the other hand, despite in vitro evidence that caspase-3 cleaves monomeric tau at Asp(421), to date, this truncation has not been demonstrated to be executed by this protease in polymeric tau entities. We determined that Asp(421) truncation can be produced by caspase-3 in oligomeric and multimeric complexes of recombinant full-length tau in isolated native tau filaments in vitro and in situ in neurofibrillary tangles analyzed in fresh brain slices from AD cases. Our data suggest that generation of this pathologic Asp(421) truncation of tau in long-lasting fibrillary structures may produce further permanent toxicity for neurons in the brains of patients with AD.

Published

2013

3. Neura, nerves, nerve fibers, neurofibrils, microtubules: multidimensional routes of pain, pleasure, and voluntary action in images across the ages.

Author

Frixione E

Subjects

Animals, History, 15th Century, History, 16th Century, History, 17th Century, History, 18th Century, History, 19th Century, History, 20th Century, History, Ancient, History, Medieval, Humans, Microtubules ultrastructure, Nerve Fibers ultrastructure, Neurofibrils ultrastructure, Pain, Pleasure physiology, Psychomotor Performance physiology, Anatomy, Artistic history, Nervous System anatomy & histology

Abstract

Available records indicate that the human body has always been conceived, in different periods and cultures, as spanned by multiple channels for internal communication and coherent functioning as a unit-"meridians" in treatises of Chinese medicine, metu in Egyptian papyri, srotas in Ayurvedic Indian texts, and neura in the Western scientific heritage from ancient Greece. Unfortunately, the earliest extant figurative depictions of such pathways of general control, complementary to the blood vessels, are late medieval copies of old crude sketches that attempted to show the main anatomico-physiological systems. The scarcity of adequate illustrations was more than compensated in the Renaissance, when the efforts of both artists and anatomists for the first time produced basically correct renditions of the human nervous system and many other bodily structures. As attention was next focused on microscopic structure as a requisite to understand physiological mechanisms, during the Enlightenment the nerves were revealed to consist of numerous thin tubes or fibers aligned in parallel. Improved microscopy techniques in the nineteenth century led to discovering and delineating still finer fibrils coursing along the cores of the nerve fibers themselves. Electron microscopy, developed throughout the twentieth century, recognized some of these fibrils within nerve fibers as being also tubular. All the progressive stages in understanding nerve construction, at increasingly more detailed scales, have been accompanied by technological advances and by debate about the structure and function relationship. And every step has been a source of amazing imagery., (© 2013 Elsevier B.V. All rights reserved.)

Published

2013

4. Histomorphological study of myelinated nerve fibres in the periodontal ligament of human canine.

Author

Huang Y, Corpas LS, Martens W, Jacobs R, and Lambrichts I

Subjects

Aged, Alveolar Process innervation, Axons ultrastructure, Blood Vessels innervation, Cadaver, Collagen ultrastructure, Humans, Immunohistochemistry, Male, Mechanoreceptors ultrastructure, Neurofibrils ultrastructure, Periodontal Ligament blood supply, Tooth Apex innervation, Tooth Root innervation, Cuspid innervation, Nerve Fibers, Myelinated ultrastructure, Periodontal Ligament innervation

Abstract

Objective: This study aims to describe the human periodontal ligament (PDL) using serial sections, with a focus on mechanoreceptor distribution and morphology., Materials and Methods: One permanent lower canine with surrounding PDL and alveolar bone tissues was retrieved from a human cadaver. After being embedded into paraffin block, the canine was horizontally cut in 6 μm thick serial sections. At root levels of 0.3, 1.5, 3, 4.5 and 6 mm from the apex, five slices each level were evaluated. Immunocytochemisty was performed on the same serial sections, enabling a more reliable description of neural structures., Results: The distribution of myelinated fibres varied from apical to coronal level, with a total number of 38 at 0.3 mm from the apex, 25 at 1.5 mm, 25 at 3 mm, 31 at 4.5 mm and 32 at 6 mm. At all times, mesial and buccal regions were typically more densely innervated (p < 0.01) except at the 3 mm level. The average density of myelinated nerve fibres increased by arriving closer to the apex. However, the average diameter did not show any significant differences amongst quadrants or root levels (p > 0.05). The average diameter of myelinated fibres varied between 5.3-7.8 μm. Grouped myelinated axons were twice as common as isolated ones, with the innervation being rather close to the alveolar bone. Isolated myelinated axons showed a tendency to group around large blood vessels., Conclusion: The present results add to the understanding of human PDL innervation, indicating dense innervations by myelinated nerve fibres in close proximity to collagen fibres and alveolar bone. It also reveals that apical as well as mesial and buccal sites of the human canine are more densely innervated.

Published

2011

5. Axon cytoskeleton ultrastructure in chronic inflammatory demyelinating polyneuropathy.

Author

Fressinaud C and Dubas F

Subjects

Aged, Axons pathology, Biopsy, Case-Control Studies, Female, GAP-43 Protein metabolism, Humans, Male, Microtubules ultrastructure, Middle Aged, Myelin Sheath ultrastructure, Neurofibrils ultrastructure, Polyradiculoneuropathy, Chronic Inflammatory Demyelinating metabolism, Severity of Illness Index, Axons ultrastructure, Cytoskeleton ultrastructure, Polyradiculoneuropathy, Chronic Inflammatory Demyelinating pathology

Abstract

Introduction: To detail the extent and pattern of axon cytoskeleton alterations in chronic inflammatory demyelinating polyneuropathy (CIDP)., Methods: Nerve biopsies from 7 cases of CIDP, including 4 cases with severe fiber loss, were compared with 5 controls by morphometric transmission electron microscopy (TEM)., Results: Despite demyelination of single fibers, myelin ultrastructure was otherwise normal. Contrary to immunolabeling, TEM revealed a decrease in neurofilament (NF) density in every case, although there were pronounced variations among fibers even in the same sample. The NF decrease reached the same extent in large- and small-diameter fibers. It was observed in normally myelinated fibers, suggesting they were demyelinated at a distance from the section. Minimal inter-NF distance increased roughly inversely to NF density. Microtubules increased in 3 cases previously characterized by increased growth-associated protein (GAP-43) immunolabeling., Conclusion: These data demonstrate the severity and constancy of axonal lesions, and especially of NF, in residual fibers in our cases of CIDP., (Copyright © 2011 Wiley Periodicals, Inc.)

Published

2011

6. Cajal's second great battle for the neuron doctrine: the nature and function of neurofibrils.

Author

Frixione E

Subjects

Animals, Central Nervous System physiology, Cytoskeleton physiology, Cytoskeleton ultrastructure, History, 19th Century, History, 20th Century, Humans, Interdisciplinary Communication, Models, Theoretical, Nerve Net physiology, Nerve Net ultrastructure, Neuroanatomy methods, Neurofibrils physiology, Neurons physiology, Staining and Labeling history, Staining and Labeling methods, Central Nervous System ultrastructure, Nervous System Physiological Phenomena, Neuroanatomy history, Neurofibrils ultrastructure, Neurons ultrastructure

Abstract

One hundred years ago, a novel kind of reticularism threatened to displace the neuron doctrine as the established model of functional organization of the nervous system. The challenging paradigm, championed by Stephan von Apáthy and Albrecht Bethe, held that nerve impulses propagate along neurofibrils connected in a continuous network throughout all nerve cells. Santiago Ramón y Cajal, a leading figure in the conception of the neuron doctrine, headed again the battle against this return of reticularism. Dissatisfied with the available staining techniques, he devised the "reduced silver nitrate method" that even Camillo Golgi recognized as the best at the time for revealing the neurofibrils. In 1904 Cajal already published over a dozen papers in three languages describing neurofibril distributions in the nervous systems of diverse vertebrates and invertebrates, under both normal and experimental conditions. Next he investigated the involvement of neurofibrils in the process of nerve regeneration. This unprecedented survey led him to the conclusion that the neurofibrils are linear "colonies" of particles constituting a semi-solid, dynamic internal skeleton of the nerve cell. Apáthy reacted with a long invective paper that Cajal had no choice but acknowledging. His comprehensive reply, published in 1908, meant the effective end of the renewed reticularist campaign against the neuron doctrine. Along the way, a visionary and today almost forgotten chapter in the history of the cytoskeleton had also been written.

Published

2009

7. Acute and delayed implantation of positively charged 2-hydroxyethyl methacrylate scaffolds in spinal cord injury in the rat.

Author

Hejcl A, Urdzikova L, Sedy J, Lesny P, Pradny M, Michalek J, Burian M, Hajek M, Zamecnik J, Jendelova P, and Sykova E

Subjects

Animals, Axons pathology, Axons physiology, Biocompatible Materials chemistry, Connective Tissue pathology, Cysts pathology, Disease Models, Animal, Guided Tissue Regeneration, Hydrogels chemistry, Male, Methacrylates chemistry, Nerve Regeneration physiology, Neurofibrils ultrastructure, Paraplegia physiopathology, Rats, Rats, Wistar, Schwann Cells pathology, Spinal Cord blood supply, Spinal Cord pathology, Time Factors, Wound Healing physiology, Biocompatible Materials therapeutic use, Hydrogels therapeutic use, Methacrylates therapeutic use, Spinal Cord Injuries surgery, Tissue Scaffolds

Abstract

Object: Hydrogels are nontoxic, chemically inert synthetic polymers with a high water content and large surface area that provide mechanical support for cells and axons when implanted into spinal cord tissue., Methods: Macroporous hydrogels based on 2-hydroxyethyl methacrylate (HEMA) were prepared by radical copolymerization of monomers in the presence of fractionated NaCl particles. Male Wistar rats underwent complete spinal cord transection at the T-9 level. To bridge the lesion, positively charged HEMA hydrogels were implanted either immediately or 1 week after spinal cord transection; control animals were left untreated. Histological evaluation was performed 3 months after spinal cord transection to measure the volume of the pseudocyst cavities and the ingrowth of tissue elements into the hydrogels., Results: The hydrogel implants adhered well to the spinal cord tissue. Histological evaluation showed ingrowth of connective tissue elements, blood vessels, neurofilaments, and Schwann cells into the hydrogels. Morphometric analysis of lesions showed a statistically significant reduction in pseudocyst volume in the treated animals compared with controls and in the delayed treatment group compared with the immediate treatment group (p < 0.001 and p < 0.05, respectively)., Conclusions: Positively charged HEMA hydrogels can bridge a posttraumatic spinal cord cavity and provide a scaffold for the ingrowth of regenerating axons. The results indicate that delayed implantation can be more effective than immediate reconstructive surgery.

Published

2008

8. Amyloidosis in transgenic mice expressing murine amyloidogenic apolipoprotein A-II (Apoa2c).

Author

Ge F, Yao J, Fu X, Guo Z, Yan J, Zhang B, Zhang H, Tomozawa H, Miyazaki J, Sawashita J, Mori M, and Higuchi K

Subjects

Amyloidosis pathology, Animals, Apolipoprotein A-II ultrastructure, Cloning, Molecular, Disease Models, Animal, Immunohistochemistry, Mice, Mice, Inbred Strains, Mice, Transgenic, Microscopy, Electron, Transmission, Neurofibrils pathology, Protein Biosynthesis, Tissue Distribution, Amyloid metabolism, Amyloid ultrastructure, Amyloidosis metabolism, Apolipoprotein A-II biosynthesis, Neurofibrils ultrastructure

Abstract

In mice, apolipoprotein A-II (apoA-II) self-associates to form amyloid fibrils (AApoAII) in an age-associated manner. We postulated that the two most important factors in apoA-II amyloidosis are the Apoa2(c) allele, which codes for the amyloidogenic protein APOA2C (Gln5, Ala38) and transmission of amyloid fibrils. To characterize further the contribution of the Apoa2(c) allele to amyloidogenesis and improve detection of amyloidogenic materials, we established transgenic mice that overexpress APOA2C protein under the cytomegalovirus (CMV) immediate early gene (CMV-IE) enhancer/chicken beta promoter. Compared to transgene negative (Tg(-/-)) mice that express apoA-II protein mainly in the liver, mice homozygous (Tg(+/+)) and heterozygous (Tg(+/-)) for the transgene express a high level of apoA-II protein in many tissues. They also have higher plasma concentrations of apoA-II, higher ratios of ApoA-II/apolipoprotein A-I (ApoA-I) and higher concentrations of high-density lipoprotein (HDL) cholesterol. Following injection of AApoAII fibrils into Tg(+/+) mice, amyloid deposition was observed in the testis, liver, kidney, heart, lungs, spleen, tongue, stomach and intestine but not in the brain. In Tg(+/+) mice, but not in Tg(-/-) mice, amyloid deposition was induced by injection of less than 10(-8) mug AApoAII fibrils. Furthermore, deposition in Tg(+/+) mice occurred more rapidly and to a greater extent than in Tg(-/-) mice. These studies indicate that increased levels of APOA2C protein lead to earlier and greater amyloid deposition and enhanced sensitivity to the transmission of amyloid fibrils in transgenic mice. This transgenic mouse model should prove valuable for studies of amyloidosis.

Published

2007

9. Vitamin A potently destabilizes preformed alpha-synuclein fibrils in vitro: implications for Lewy body diseases.

Author

Ono K and Yamada M

Subjects

Antioxidants chemistry, Antioxidants pharmacology, Benzothiazoles, Coenzymes, Humans, Microscopy, Atomic Force, Microscopy, Electron, Microscopy, Fluorescence, Neurofibrils metabolism, Neurofibrils ultrastructure, Neuroprotective Agents pharmacology, Thiazoles, Ubiquinone analogs & derivatives, Ubiquinone chemistry, Ubiquinone pharmacology, Vitamin A pharmacology, Vitamins chemistry, Vitamins pharmacology, alpha-Synuclein chemistry, alpha-Synuclein metabolism, beta Carotene chemistry, beta Carotene pharmacology, Lewy Body Disease metabolism, Neurofibrils drug effects, Neuroprotective Agents chemistry, Parkinson Disease metabolism, Vitamin A chemistry, alpha-Synuclein drug effects

Abstract

Alpha-synuclein (alphaS) is the major component of the filamentous inclusions that constitute defining characteristics of Lewy body diseases (LBD) and multiple system atrophy (MSA). Clinically, antioxidant vitamins, such as vitamin E and the vitamin-like substance coenzyme Q10, have been used in the treatment of LBD with some efficacy. Using fluorescence spectroscopy with thioflavin S, electron microscopy and atomic force microscopy, here we examined the effects of ten antioxidant vitamins and vitamin-like substances, vitamin A (retinol, retinal and retinoic acid), beta-carotene, vitamins B2, B6, C, E, coenzyme Q10 and alpha-lipoic acid, on the formation of alphaS fibrils (falphaS) and on preformed falphaS. Among them, vitamin A, beta-carotene and coenzyme Q10 dose-dependently inhibited the formation of falphaS. Moreover, they also dose-dependently destabilized preformed falphaS. With such potent anti-fibrillogenic as well as fibril-destabilizing activities, these compounds could be useful in the treatment and prevention of LBD and MSA.

Published

2007

10. Tau-dependent microtubule disassembly initiated by prefibrillar beta-amyloid.

Author

King ME, Kan HM, Baas PW, Erisir A, Glabe CG, and Bloom GS

Subjects

Alzheimer Disease pathology, Animals, COS Cells, Chlorocebus aethiops, Humans, Mice, Microscopy, Fluorescence, Neurofibrils ultrastructure, Phosphorylation drug effects, Protein Structure, Quaternary drug effects, Rats, tau Proteins chemistry, Amyloid beta-Peptides pharmacology, Microtubules drug effects, Microtubules metabolism, Neurofibrils drug effects, Peptide Fragments pharmacology, tau Proteins metabolism

Abstract

Alzheimer's Disease (AD) is defined histopathologically by extracellular beta-amyloid (Abeta) fibrils plus intraneuronal tau filaments. Studies of transgenic mice and cultured cells indicate that AD is caused by a pathological cascade in which Abeta lies upstream of tau, but the steps that connect Abeta to tau have remained undefined. We demonstrate that tau confers acute hypersensitivity of microtubules to prefibrillar, extracellular Abeta in nonneuronal cells that express transfected tau and in cultured neurons that express endogenous tau. Prefibrillar Abeta42 was active at submicromolar concentrations, several-fold below those required for equivalent effects of prefibrillar Abeta40, and microtubules were insensitive to fibrillar Abeta. The active region of tau was localized to an N-terminal domain that does not bind microtubules and is not part of the region of tau that assembles into filaments. These results suggest that a seminal cell biological event in AD pathogenesis is acute, tau-dependent loss of microtubule integrity caused by exposure of neurons to readily diffusible Abeta.

Published

2006

11. Polymerization of hyperphosphorylated tau into filaments eliminates its inhibitory activity.

Author

Alonso Adel C, Li B, Grundke-Iqbal I, and Iqbal K

Subjects

3T3 Cells, Alzheimer Disease metabolism, Animals, Biopolymers chemistry, Biopolymers metabolism, Cells, Cultured, Humans, Mice, Microtubules metabolism, Models, Biological, Neurofibrils ultrastructure, Phosphorylation, Protein Binding, Protein Structure, Quaternary, tau Proteins ultrastructure, Alzheimer Disease pathology, Neurofibrils chemistry, Neurofibrils metabolism, tau Proteins chemistry, tau Proteins metabolism

Abstract

Accumulation of abnormally hyperphosphorylated tau (P-tau) in the form of tangles of paired helical filaments and/or straight filaments is one of the hallmarks of Alzheimer's disease (AD) and other tauopathies. P-tau is also found unpolymerized in AD. Although the cognitive decline is known to correlate with the degree of neurofibrillary pathology, whether the formation of filaments or the preceding abnormal hyperphosphorylation of tau is the inhibitory entity that leads to neurodegeneration has been elusive. We have previously shown that cytosolic abnormally hyperphosphorylated tau in AD brain (AD P-tau) sequesters normal tau (N-tau), microtubule-associated protein (MAP) 1, and MAP2, which results in the inhibition of microtubule assembly and disruption of microtubules. Here, we show that polymerization of AD P-tau into filaments inhibits its ability to bind N-tau and as well as the ability to inhibit the assembly of tubulin into microtubules in vitro and in the regenerating microtubule system from cultured cells. Like AD P-tau, the in vitro abnormally hyperphosphorylated recombinant brain N-tau binds N-tau and loses this binding activity on polymerization into filaments. Dissociation of the hyperphosphorylated N-tau filaments by ultrasonication restores its ability to bind N-tau. These findings suggest that the nonfibrillized P-tau is most likely the responsible entity for the disruption of microtubules in neurons in AD. The efforts in finding a therapeutic intervention for tau-induced neurodegeneration need to be directed either to prevent the abnormal hyperphosphorylation of this protein or to neutralize its binding to normal MAPs, rather than to prevent its aggregation into filaments.

Published

2006

12. The fate of axons subjected to traumatic ultrastructural (neurofilament) compaction: an electron-microscopic study.

Author

Gallyas F, Pál J, Farkas O, and Dóczi T

Subjects

Animals, Craniocerebral Trauma physiopathology, Microscopy, Electron, Transmission, Myelin Sheath pathology, Nerve Degeneration pathology, Rats, Rats, Wistar, Silver, Axons ultrastructure, Craniocerebral Trauma pathology, Neurofibrils ultrastructure

Abstract

By means of a new head-injury apparatus, a 0.75-mm-deep depression was produced momentarily at a predetermined site of the rat calvaria. This immediately evoked ultrastructural (neurofilament) compaction in many myelinated axon segments in layers IV and V of the neocortex under the impact site. The affected axon segments run quasi-parallel to the brain surface in a diffuse distribution among normal axons. Other kinds of damage to the brain tissue were insignificant; the conditions were therefore favorable for investigation of the fate of the compacted axons. Quantitative analysis of the findings on groups of ten rats that were sacrificed either immediately after the head injury or following a 1 day or a 1 week survival period showed that around 50% of the compacted axons recovered in 1 day, and a further less than 10% did so in 1 week. Electron microscopy revealed that the non-recovering compacted axons underwent a sequence of degenerative morphological changes including homogenization, fragmentation and resorption of the fragments. However, the myelin sheaths around these degenerating axons remained apparently unchanged even in the long-surviving rats, and hardly any phagocytotic cells were encountered. On the other hand, many such myelin sheaths contained axolemma-bound, normal-looking axoplasm besides the above morphological signs of axon-degeneration. It is concluded that the non-recovering compacted axons undergo an uncommon (non-Wallerian) kind of degeneration, which is mostly reversible.

Published

2006

13. Non-steroidal anti-inflammatory drugs have anti-amyloidogenic effects for Alzheimer's beta-amyloid fibrils in vitro.

Author

Hirohata M, Ono K, Naiki H, and Yamada M

Subjects

Alzheimer Disease pathology, Amyloid beta-Peptides metabolism, Cells, Cultured, Dose-Response Relationship, Drug, Humans, Hydrogen-Ion Concentration, Kinetics, Microscopy, Electron, Microscopy, Fluorescence, Neurofibrils drug effects, Neurofibrils ultrastructure, Alzheimer Disease metabolism, Amyloid beta-Peptides antagonists & inhibitors, Amyloidosis pathology, Amyloidosis prevention & control, Anti-Inflammatory Agents, Non-Steroidal pharmacology, Neurofibrils metabolism

Abstract

The pathogenesis of Alzheimer's disease (AD) is characterized by cerebral deposits of amyloid beta-peptides (A beta) and neurofibrillary tangles which are surrounded by inflammatory cells. Long-term use of non-steroidal anti-inflammatory drugs (NSAIDs) reduces the risk of developing AD and delays the onset of the disease. In the present study, we used fluorescence spectroscopy with thioflavin T and electron microscopy to examine the effects of NSAIDs such as ibuprofen, aspirin, meclofenamic acid sodium salt, diclofenac sodium salt, ketoprofen, flurbiprofen, naproxen, sulindac sulfide and indomethacin on the formation, extension, and destabilization of beta-amyloid fibrils (fA beta) at pH 7.5 at 37 degrees C in vitro. All examined NSAIDs dose-dependently inhibited formation of fA beta from fresh A beta(1-40) and A beta(1-42), as well as their extension. Moreover, these NSAIDs dose-dependently destabilized preformed fA betas. The overall activity of the molecules examined was in the following order: ibuprofen approximately sulindac sulfide >or= meclofenamic acid sodium salt>aspirin approximately ketoprofen >or= flurbiprofen approximately diclofenac sodium salt>naproxen approximately indomethacin. Although the mechanisms by which these NSAIDs inhibit fA beta formation from A beta, and destabilize preformed fA beta in vitro are still unclear, NSAIDs may be promising for the prevention and treatment of AD.

Published

2005

14. Identification of synaptic plasma membrane proteins co-precipitated with fibrillar beta-amyloid peptide.

Author

Verdier Y, Huszár E, Penke B, Penke Z, Woffendin G, Scigelova M, Fülöp L, Szucs M, Medzihradszky K, and Janáky T

Subjects

Amyloid beta-Peptides isolation & purification, Animals, Brain cytology, Brain metabolism, Cell Membrane ultrastructure, Chemical Precipitation, Chromatography, High Pressure Liquid methods, Electrophoresis, Polyacrylamide Gel methods, Gas Chromatography-Mass Spectrometry methods, Male, Microscopy, Electron, Transmission methods, Neurofibrils ultrastructure, Peptide Fragments isolation & purification, Protein Binding physiology, Rats, Rats, Wistar, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods, Synapses ultrastructure, Synaptosomes metabolism, Synaptosomes ultrastructure, beta-Crystallins metabolism, Amyloid beta-Peptides metabolism, Cell Membrane metabolism, Membrane Proteins isolation & purification, Neurofibrils metabolism, Peptide Fragments metabolism, Synapses metabolism

Abstract

The beta-amyloid peptide that is overproduced in Alzheimer's disease rapidly forms fibrils, which are able to interact with various molecular partners. This study aimed to identify abundant synaptosomal proteins binding to the fibrillar beta-amyloid (fAbeta) 1-42. Triton X-100-soluble proteins were extracted from the rat synaptic plasma membrane fraction. Interacting proteins were isolated by co-precipitation with fAbeta, or with fibrillar crystallin as a negative control. Protein identification was accomplished (1) by separating the tryptically digested peptides of the protein pellet by one-dimensional reversed-phase HPLC and analysing them using an ion-trap mass spectrometer with electrospray ionization; and (2) by subjecting the precipitated proteins to gel electrophoretic fractionation, in-gel tryptic digestion and to matrix-assisted laser desorption/ionization time-of-flight mass measurements and post-source decay analysis. Six different synaptosomal proteins co-precipitated with fAbeta were identified by both methods: vacuolar proton-pump ATP synthase, glyceraldehyde-3-phosphate dehydrogenase, synapsins I and II, beta-tubulin and 2',3'-cyclic nucleotide 3'-phosphodiesterase. Most of these proteins have already been associated with Alzheimer's disease, and the biological and pathophysiological significance of their interaction with fAbeta is discussed.

Published

2005

15. In vitro model of neurotoxicity of Abeta 1-42 and neuroprotection by a pentapeptide: irreversible events during the first hour.

Author

Datki Z, Papp R, Zádori D, Soós K, Fülöp L, Juhász A, Laskay G, Hetényi C, Mihalik E, Zarándi M, and Penke B

Subjects

Alzheimer Disease pathology, Amyloid beta-Peptides chemistry, Cell Line, Tumor, Humans, Microscopy, Electron, Scanning, Nerve Tissue Proteins drug effects, Nerve Tissue Proteins metabolism, Neurofibrils drug effects, Neurofibrils ultrastructure, Neurotoxins toxicity, Phosphorylation, Time Factors, Amyloid beta-Peptides toxicity, Peptide Fragments therapeutic use

Abstract

The cell biology of Alzheimer's disease (AD) is characterized mainly by the neurodegeneration caused by the beta-amyloid (Abeta) peptides and by the formation of neurofibrillary tangles. The initial events of neurodegeneration in the brain tissue include synaptic dysfunction and axonopathy. Abeta-induced axonopathy and neurite degeneration were studied in vitro on differentiated human-derived neurotypic SH-SY5Y cells. Different methods were used to investigate the mechanism of action of aggregated Abeta on neuroblastoma cells. Abeta 1-42 aggregated for 1 h induced irreversible changes in the neurite morphology. Change of tau hyperphosphorylation and cell viability (cytoplasmic redox state and active membrane uptake) was irreversible during the first hour after the addition of Abeta 1-42 to the cells. These rapid events indicate that Abeta might induce neurodegeneration even at an early stage of Abeta-cell contact. A novel pentapeptide LPYFD-amide, an analog of Soto's LPFFD, significantly decreased neurite degeneration, tau aggregation, and cell viability reduction induced by Abeta 1-42.

Published

2004

16. Vitamin A exhibits potent antiamyloidogenic and fibril-destabilizing effects in vitro.

Author

Ono K, Yoshiike Y, Takashima A, Hasegawa K, Naiki H, and Yamada M

Subjects

Amyloid beta-Peptides biosynthesis, Antioxidants pharmacology, Benzothiazoles, Cell Line, Dose-Response Relationship, Drug, Humans, Kinetics, Microscopy, Electron, Molecular Structure, Neurofibrils metabolism, Neurofibrils ultrastructure, Retinaldehyde pharmacology, Thiazoles, Tretinoin pharmacology, beta Carotene pharmacology, Alzheimer Disease metabolism, Amyloid beta-Peptides antagonists & inhibitors, Neurofibrils drug effects, Vitamin A pharmacology, Vitamins pharmacology

Abstract

Cerebral deposition of amyloid beta-peptide (Abeta) in the brain is an invariant feature of Alzheimer disease (AD). Plasma or cerebrospinal fluid concentrations of antioxidant vitamins and carotenoids, such as vitamins A, C, E, and beta-carotene, have been reported to be lower in AD patients, and these vitamins clinically have been demonstrated to slow the progression of dementia. In this study, we used fluorescence spectroscopy with thioflavin T (ThT) and electron microscopy to examine the effects of vitamin A (retinol, retinal, and retinoic acid), beta-carotene, and vitamins B2, B6, C, and E on the formation, extension, and destabilization of beta-amyloid fibrils (fAbeta) in vitro. Among them, vitamin A and beta-carotene dose-dependently inhibited formation of fAbeta from fresh Abeta, as well as their extension. Moreover, they dose-dependently destabilized preformed fAbetas. The overall activity of the molecules examined was in the order of retinol = retinal > beta-carotene > retinoic acid. Although the exact mechanisms are still unclear, vitamins A and beta-carotene could be key molecules for the prevention and therapy of AD.

Published

2004

17. Genetic heterogeneity in giant axonal neuropathy: an Algerian family not linked to chromosome 16q24.1.

Author

Tazir M, Vallat JM, Bomont P, Zemmouri R, Sindou P, Assami S, Nouioua S, Hammadouche T, Grid D, and Koenig M

Subjects

Adolescent, Algeria, Axons ultrastructure, Child, Chromosome Mapping, Demyelinating Diseases genetics, Demyelinating Diseases pathology, Demyelinating Diseases physiopathology, Electrophysiology, Family, Female, Genetic Heterogeneity, Genetic Linkage, Humans, Male, Microscopy, Electron, Neurofibrils ultrastructure, Pedigree, Axons pathology, Chromosomes, Human, Pair 16 genetics, Nervous System Diseases genetics

Abstract

Giant axonal neuropathy is a rare severe autosomal recessive childhood disorder affecting both the peripheral nerves and the central nervous system. Peripheral nerves characteristically show giant axonal swellings filled with neurofilaments. The giant axonal neuropathy gene was localised by homozygosity mapping to chromosome 16q24.1 and identified as encoding a novel, ubiquitously expressed cytoskeletal protein named gigaxonin.We describe a consanguineous Algerian family with three affected sibs aged 16, 14 and 12 years who present a mild demyelinating sensory motor neuropathy, hypoacousia and kyphoscoliosis which was moderate in the two elder patients, severe in the third one, with no sign of central nervous system involvement and normal cerebral magnetic resonance imaging. This clinical picture is different from the classical severe form, with kinky hairs and early onset of central nervous system involvement and from the less severe form, with protracted course and late involvement of central nervous system. Nerve biopsy showed a moderate loss of myelinated fibers and several giant axons with thin or absent myelin, filled with neurofilaments. This neuropathological aspect is similar to the previously described families linked to the gigaxonin gene. Genetic study in this family showed absence of linkage to chromosome 16q24.1, indicating for the first time, a genetic heterogeneity in giant axonal neuropathy. We propose to call this form of giant axonal neuropathy giant axonal neuropathy 2, and to use the name of giant axonal neuropathy 1 for the form linked to 16q24.1.

Published

2002

18. Laminin affects polymerization, depolymerization and neurotoxicity of Abeta peptide.

Author

Morgan C, Bugueño MP, Garrido J, and Inestrosa NC

Subjects

Amyloid beta-Peptides ultrastructure, Animals, Cells, Cultured, Dose-Response Relationship, Drug, Hippocampus cytology, Humans, Kinetics, Mice, Neurofibrils ultrastructure, Neurons cytology, Neurotoxins antagonists & inhibitors, Peptide Fragments chemistry, Peptide Fragments ultrastructure, Rats, Amyloid beta-Peptides toxicity, Laminin pharmacology, Neurons drug effects, Neuroprotective Agents pharmacology, Peptide Fragments pharmacology, Peptide Fragments toxicity, Polymers metabolism

Abstract

Amyloid deposition in Alzheimer fibrils forms neurotoxic senile plaques in a process that may be modulated by associated proteins. In this work we demonstrate the ability of laminin-1 and laminin-2 to inhibit fibril formation and toxicity on cultured rat hippocampal neurons. We confirm that the laminin-1-derived peptide YFQRYLI inhibits efficiently both fibril formation and neurotoxicity and show that the IKVAV peptide inhibits amyloid neurotoxicity despite its slight inhibition of fibril formation. On other hand, laminin-1 induces disaggregation of preformed fibrils in vitro, characterized as a progressive disassembly of fibrils into protofibrils and further clearance of these latter species, leading to a continual inhibition of amyloid neurotoxicity.

Published

2002

19. Fibrillar inclusions and motor neuron degeneration in transgenic mice expressing superoxide dismutase 1 with a disrupted copper-binding site.

Author

Wang J, Xu G, Gonzales V, Coonfield M, Fromholt D, Copeland NG, Jenkins NA, and Borchelt DR

Subjects

Animals, Benzothiazoles, Binding Sites, Disease Models, Animal, Female, Histidine chemistry, Humans, Male, Mice, Mice, Inbred C3H, Mice, Inbred C57BL, Mice, Transgenic, Motor Neuron Disease enzymology, Motor Neuron Disease pathology, Motor Neurons pathology, Nerve Tissue Proteins chemistry, Neurofibrils ultrastructure, Protein Folding, Spinal Cord pathology, Structure-Activity Relationship, Superoxide Dismutase chemistry, Superoxides metabolism, Thiazoles analysis, Amino Acid Substitution, Copper metabolism, Motor Neuron Disease genetics, Mutation, Missense, Nerve Tissue Proteins genetics, Superoxide Dismutase genetics

Abstract

Mutations in Cu/Zn superoxide dismutase 1 (SOD1) have been linked to dominantly inherited forms of amyotrophic lateral sclerosis (FALS). To test the hypothesis that the toxicity of mutant SOD1 originates in Cu(2+)-mediated formation of toxic radicals, we generated transgenic mice that express human SOD1 that encodes disease-linked mutations at two of the four histidine residues that are crucial for the coordinated binding of copper (H46R/H48Q). We demonstrate that mice expressing this mutant, which possesses little or no superoxide scavenging activity, develop motor neuron disease. Hence, mutations in SOD1 that disrupt the copper-binding site do not eliminate toxicity. We note that the pathology of the H46R/H48Q mice is dominated by fibrillar (Thioflavin-S-positive) inclusions and that similar inclusions were evident in mouse models that express the G37R, G85R, and G93A variants of human SOD1. Overall, our data are consistent with the hypothesis that the aberrant folding/aggregation of mutant SOD1 is a prominent feature in the pathogenesis of motor neuron disease.

Published

2002

20. Imaging real-time aggregation of amyloid beta protein (1-42) by atomic force microscopy.

Author

Parbhu A, Lin H, Thimm J, and Lal R

Subjects

Air, Amyloid beta-Peptides ultrastructure, Calcium metabolism, Edetic Acid metabolism, Edetic Acid pharmacology, Neurofibrils metabolism, Neurofibrils ultrastructure, Peptide Fragments ultrastructure, Protein Conformation, Sodium Chloride, Time Factors, Water, Zinc metabolism, Zinc pharmacology, Amyloid beta-Peptides metabolism, Microscopy, Atomic Force, Peptide Fragments metabolism

Abstract

Amyloid beta protein (AbetaP) is the major fibrillar constituent of senile plaques. However, no causative role for AbetaP-fibers in Alzheimer's disease (AD) pathology is established. Globular AbetaPs are continuously released during normal cellular metabolism at pico- to nano-molar concentration. We used atomic force microscopy (AFM) to examine aggregation of freshly prepared AbetaP(1-42) and to examine the role of AbetaP concentration, imaging medium (air, water, or PBS) and agonists/antagonists on AbetaP-fibrillogenesis. At even very high and non-physiological AbetaP concentrations, 24-48 h of real-time AFM imaging (a) in water show only multiple layers of globular aggregates and no fibrils and (b) in PBS show mainly the globular structures and some short fibrils. On-line addition of Zn, an agonist for AbetaP-fibrillogenesis, induced a slow but non-fibrillar aggregation of globular AbetaPs. EDTA, a chelator of Zn and calcium (a modulator of AbetaP-mediated toxicity) induced a reversible change in the Zn-mediated aggregation. These results strongly suggest that no AbetaP-fibers are formed for the physiologically relevant concentration and thus the plaque-associated fibers may not account for the AD pathophysiology.

Published

2002

21. ADDLs & protofibrils--the missing links?

Author

Klein WL

Subjects

Alzheimer Disease pathology, Humans, Neurofibrils metabolism, Neurofibrils ultrastructure, Alzheimer Disease metabolism, Amyloid metabolism, Amyloid beta-Peptides metabolism, Neurofibrils pathology

Published

2002

22. Structure and location of amyloid beta peptide chains and arrays in Alzheimer's disease: new findings require reevaluation of the amyloid hypothesis and of tests of the hypothesis.

Author

Rosenblum WI

Subjects

Alzheimer Disease pathology, Amyloid beta-Peptides chemistry, Humans, Neurofibrils metabolism, Neurofibrils pathology, Neurofibrils ultrastructure, Alzheimer Disease metabolism, Amyloid metabolism, Amyloid beta-Peptides metabolism

Abstract

New in situ high resolution electronmicroscopic examination of amyloid fibrils in situ indicate that in Alzheimer's disease these fibrils are not simply long chains of self aggregated amyloid beta peptide. The amyloid beta is not only associated with P protein and glycans, as was well known from previous immunohistologic studies, but is arranged in the form of short chains at right angles to a P protein backbone with the glycans wrapped around that backbone. These findings suggest that the hypothesis causally relating simple, fibrillar amyloid beta to Alzheimer's disease must be reevaluated since such simple fibrils may be absent, or not the major form of the amyloid beta in the brain. Other data shows that shorter multimers, so-called protofibrils, or dimers of amyloid beta or molecules cleaved from it can be highly toxic. Some of these may be in the soluble amyloid beta fraction. Shorter multimers or dimers of amyloid beta, either extra or intracellular, may be the real links between amyloid beta production and Alzheimer's disease. Toxicity studies employing fibrillar amyloid beta may not be relevant, even if they produce lesions, because they do not employ amyloid beta in the form in which it actually exists in the Alzheimer brain. Studies of treatments designed to remove fibrils or to prevent their formation may be ineffective or suboptimal in effectiveness because they do not reduce the relevant amyloid burden and/or fail to alter the arrangement of shorter multimers of amyloid beta around its P-protein and glycan core.

Published

2002

23. [Modification of the Bilshovsky method for studies of nerve tissue paraffin sections].

Author

Sukhanov AV and Vakulin GM

Subjects

Alzheimer Disease pathology, Humans, Male, Nerve Tissue ultrastructure, Neurofibrils ultrastructure, Paraffin Embedding, Thalamus ultrastructure, Nerve Tissue cytology

Abstract

The Bilshovsky method is often used for studies of the morphology of neuronal fibrillar system. The classical variant of this method requires sections made with a freezing microtome, which is sometimes inconvenient. Preparation of paraffin sections often gives unsatisfactory results. The authors managed to overcome this deficiency. Their modification consists in the following: after deparaffinization of paraffin sections glued to the slides they are repeatedly fixed in warm formalin and then treated with silver nitrate with heating. This modification is easily reproducible and essentially simplifies staining; no freezing microtome is needed.

Published

2002

24. Distribution and dynamic process of neuronal cytoplasmic inclusion (NCI) in MSA: correlation of the density of NCI and the degree of involvement of the pontine nuclei.

Author

Yokoyama T, Kusunoki JI, Hasegawa K, Sakai H, and Yagishita S

Subjects

Adult, Age of Onset, Aged, Cytoplasm metabolism, Cytoplasm ultrastructure, Female, Humans, Immunohistochemistry, Inclusion Bodies metabolism, Inclusion Bodies ultrastructure, Male, Microscopy, Electron, Microscopy, Electron, Scanning, Middle Aged, Multiple System Atrophy metabolism, Multiple System Atrophy physiopathology, Nerve Tissue Proteins metabolism, Neurites metabolism, Neurites pathology, Neurites ultrastructure, Neurofibrils metabolism, Neurofibrils pathology, Neurofibrils ultrastructure, Neurofilament Proteins metabolism, Neurons metabolism, Neurons ultrastructure, Organelles metabolism, Organelles pathology, Organelles ultrastructure, Pons metabolism, Pons physiopathology, Synucleins, Ubiquitin metabolism, tau Proteins metabolism, Cytoplasm pathology, Inclusion Bodies pathology, Multiple System Atrophy pathology, Neurons pathology, Pons pathology

Abstract

MSA is a sporadic degenerative disease that occurs in striatonigral degeneration (SND), SDS and most cases of sporadic OPCA. Oligodendroglial inclusion is a hallmark of MSA. Recently there have been a small number of reports of neuronal argyrophilic inclusions. To clarify the distribution and dynamic process of neuronal cytoplasmic inclusions (NCI), 31 cases of MSA were studied using histology, immunohistochemistry, and electron microscopy. The inclusions were exclusively found in the pontine nucleus and there was a correlation between the incidence of NCI and the severity of OPCA, but not of SND. NCI were increased to some extent in the cases with moderate OPCA and decreased in number in proportion to devastation of the pontine nuclei. Immunohistochemical and ultrastructural features of NCI were virtually identical to those of glial cytoplasmic inclusions (GCI), which gives some clues to the pathogenesis of MSA. It is tempting to interpret this as NCI playing a significant role in the degenerative changes of the neurons at least in the pons. Further systematic studies on NCI in the other brain regions are necessary to elucidate the pathogenesis of neuronal degeneration in MSA.

Published

2001

25. Neurofilaments consist of distinct populations that can be distinguished by C-terminal phosphorylation, bundling, and axonal transport rate in growing axonal neurites.

Author

Yabe JT, Chylinski T, Wang FS, Pimenta A, Kattar SD, Linsley MD, Chan WK, and Shea TB

Subjects

Animals, Axons physiology, Axons ultrastructure, Cells, Cultured, Fluorescent Antibody Technique, Microscopy, Immunoelectron, Neurofibrils classification, Neurofibrils physiology, Neurofibrils ultrastructure, Phosphorylation, Amoxicillin-Potassium Clavulanate Combination therapeutic use, Biological Transport physiology, Neurites physiology, Neurofibrils metabolism

Abstract

We examined the steady-state distribution and axonal transport of neurofilament (NF) subunits within growing axonal neurites of NB2a/d1 cells. Ultrastructural analyses demonstrated a longitudinally oriented "bundle" of closely apposed NFs that was surrounded by more widely spaced individual NFs. NF bundles were recovered during fractionation and could be isolated from individual NFs by sedimentation through sucrose. Immunoreactivity toward the restrictive C-terminal phospho-dependent antibody RT97 was significantly more prominent on bundled than on individual NFs. Microinjected biotinylated NF subunits, GFP-tagged NF subunits expressed after transfection, and radiolabeled endogenous subunits all associated with individual NFs before they associated with bundled NFs. Biotinylated and GFP-tagged NF subunits did not accumulate uniformly along bundled NFs; they initially appeared within the proximal portion of the NF bundle and only subsequently were observed along the entire length of bundled NFs. These findings demonstrate that axonal NFs are not homogeneous but, rather, consist of distinct populations. One of these is characterized by less extensive C-terminal phosphorylation and a relative lack of NF-NF interactions. The other is characterized by more extensive C-terminal NF phosphorylation and increased NF-NF interactions and either undergoes markedly slower axonal transport or does not transport and undergoes turnover via subunit and/or filament exchange with individual NFs. Inhibition of phosphatase activities increased NF-NF interactions within living cells. These findings collectively suggest that C-terminal phosphorylation and NF-NF interactions are responsible for slowing NF axonal transport.

Published

2001

26. Duodenal periampullary gangliocytic paraganglioma: report of two cases with immunohistochemical and ultrastructural study.

Author

Altavilla G, Chiarelli S, and Fassina A

Subjects

Adult, Chromogranin A, Chromogranins analysis, Cytoplasmic Granules ultrastructure, Endoplasmic Reticulum ultrastructure, Female, Humans, Intestinal Mucosa pathology, Intestinal Neoplasms chemistry, Intestinal Neoplasms ultrastructure, Lysosomes ultrastructure, Male, Middle Aged, Mitochondria ultrastructure, Neurofibrils ultrastructure, Paraganglioma chemistry, Paraganglioma ultrastructure, S100 Proteins analysis, Synaptophysin analysis, Duodenum, Immunohistochemistry, Intestinal Neoplasms diagnosis, Microscopy, Electron, Paraganglioma diagnosis

Abstract

We report two cases of Gangliocytic Paraganglioma (GP) of the ampulla of Vater occurring in a 63-year-old and a 34-year-old individual. The patients were both admitted for a long history of intermittent gastrointestinal bleeding and abdominal discomfort, with no other symptoms. At endoscopy, the GP appeared as a polypoid, ulcerated mass in the ampullar region, measuring 2.5x1.8 and 2 cm, respectively. Microscopically, the tumors showed similar features and were composed of epithelial cells (more than 50%), spindle cells, and ganglion-like cells. The epithelial cells showed clear cytoplasm and formed nests (zellballen or paraganglioma-like groups), and less frequently, cords (carcinoid-like), extending to mucosa and submucosa. Ganglion cells were sparse, constantly associated with the spindle cells. Both epithelial and ganglion cells were synaptophysin, chromogranin A, and anti-neurofilament immunoreactive. The spindle cells were all S-100 positive. Ultrastructural studies revealed dark and light cells, rare elongated cellular processes, secretory granules, and fine fibrils resembling neurofilaments. The histogenesis of GP is still a matter of debate, however its neoplastic nature is supported by the occasionally reported malignant evolution.

Published

2001

27. Effects of 2,5-hexanedione on calpain-mediated degradation of human neurofilaments in vitro.

Author

Heijink E, Scholten SW, Bolhuis PA, and de Wolff FA

Subjects

Adult, Cross-Linking Reagents pharmacology, Cytoskeletal Proteins analysis, Cytoskeleton drug effects, Female, Humans, Kinetics, Male, Neuroblastoma, Neurofibrils drug effects, Neurofibrils ultrastructure, Neurofilament Proteins analysis, Sciatic Nerve drug effects, Tumor Cells, Cultured, Calpain metabolism, Cytoskeleton ultrastructure, Hexanones pharmacology, Neurotoxins pharmacology, Sciatic Nerve ultrastructure

Abstract

2,5-Hexanedione (2,5-HD), the neurotoxic metabolite of n-hexane, can structurally modify neurofilaments (NF) by pyrrole adduct formation and subsequent covalent cross-linking. 2,5-HD also induces accumulations of NF within the pre-terminal axon. We examined whether exposure of NF to 2,5-HD affected NF degradation. Two different models were used: (1) NF-enriched cytoskeletons isolated from human sciatic nerve were incubated with 2,5-HD in vitro and (2) differentiated human neuroblastoma cells (SK-N-SH) were exposed to 2, 5-HD in culture prior to isolation of cytoskeletal proteins. The cytoskeletal preparations were subsequently incubated with calpain II. The amount of NF-H and NF-L remaining after proteolysis was determined by SDS-PAGE and quantitative immunoblotting. NF-M proteolysis could not be quantified. Incubation of sciatic nerve cytoskeletal preparations with 2,5-HD resulted in cross-linking of all three NF proteins into high molecular weight (HMW) material with a range of molecular weights. Proteolysis of the NF-H and NF-L polypeptides was not affected by 2,5-HD-exposure. Degradation of the HMW material containing NF-H or NF-L was retarded when comparing with degradation of the NF-H and NF-L polypeptides, respectively, from control samples, but not as compared to the corresponding NF polypeptides from 2,5-HD-treated samples. Exposure of SK-N-SH cells to 2,5-HD also resulted in considerable cross-linking of NF. No differences were found between the proteolytic rates of NF-L and NF-H from exposed cells as compared with those subunits from control cells. Moreover, degradation of cross-linked NF-H was not different from monomeric NF-H. In conclusion, whether 2,5-HD affects calpain-mediated degradation of cross-linked NF proteins will depend on which model better reflects NF cross-linking as occurring in 2, 5-HD-induced axonopathy. However, with both models it was demonstrated that exposure of NF proteins to 2,5-HD without subsequent cross-linking is not adequate to inhibit NF proteolysis in vitro by added calpain.

Published

2000

28. Gelsolin inhibits the fibrillization of amyloid beta-protein, and also defibrillizes its preformed fibrils.

Author

Ray I, Chauhan A, Wegiel J, and Chauhan VP

Subjects

Amyloid beta-Peptides chemistry, Amyloid beta-Peptides ultrastructure, Animals, Biopolymers antagonists & inhibitors, Biopolymers chemistry, Cattle, Congo Red chemistry, Microscopy, Electron, Negative Staining, Neurofibrils chemistry, Neurofibrils ultrastructure, Peptide Fragments chemistry, Peptide Fragments ultrastructure, Protein Binding drug effects, Amyloid beta-Peptides drug effects, Gelsolin pharmacology, Neurofibrils drug effects, Peptide Fragments drug effects

Abstract

Amyloid beta-protein (Abeta) is present in soluble form in the plasma and cerebrospinal fluid (CSF) of normal people and patients with Alzheimer's disease (AD). However, in AD patients, Abeta gets fibrillized as the main constituent of amyloid plaques in the brain. Soluble synthetic Abeta also forms amyloid-like fibrils when it is allowed to age. The mechanism that prevents soluble Abeta from fibrillization in biological fluids is not clear. We recently reported that gelsolin, a secretory protein, binds to Abeta, and that gelsolin/Abeta complex is present in the plasma [V.P.S. Chauhan, I. Ray, A. Chauhan, H.M. Wisniewski, Biochem. Biophys. Res. Commun. 258 (1999) 241-246.]. We now studied the effect of gelsolin on Abeta fibrillization. Congo red staining and electron microscopic examination in negative staining of aged samples of Abeta alone and Abeta incubated with gelsolin showed that gelsolin inhibits the fibrillization of synthetic Abeta 1-40 and Abeta 1-42 at gelsolin to Abeta molar ratio of 1:40. In addition, gelsolin also defibrillized the preformed fibrils of Abeta 1-40 and Abeta 1-42 in a time-dependent manner. These results suggest that gelsolin functions as an anti-amyloidogenic protein in the plasma and CSF, where it prevents Abeta from fibrillization, and helps to maintain it in the soluble form.

Published

2000

29. Ultrastructural evidence of fibrillar beta-amyloid associated with neuronal membranes in behaviorally characterized aged dog brains.

Author

Torp R, Head E, Milgram NW, Hahn F, Ottersen OP, and Cotman CW

Subjects

Animals, Axons metabolism, Axons ultrastructure, Blood Vessels metabolism, Blood Vessels ultrastructure, Brain cytology, Brain ultrastructure, Cell Membrane metabolism, Cerebrovascular Circulation, Dendrites metabolism, Dendrites ultrastructure, Dogs, Female, Male, Microscopy, Electron, Neurofibrils ultrastructure, Amyloid beta-Peptides metabolism, Behavior, Animal physiology, Brain metabolism, Neurofibrils metabolism, Neurons metabolism

Abstract

The aged dog brain accumulates beta-amyloid in the form of diffuse senile plaques, which provides a potentially useful in vivo model system for studying the events surrounding the deposition of beta-amyloid. We used postembedding immunocytochemistry at the electron microscopic level to determine the subcellular distribution of beta-amyloid 1-40 and beta-amyloid 1-42 peptides in the prefrontal and parietal cortex of behaviorally characterized dogs ranging in age from one to 17 years. Immunogold particles signaling beta-amyloid 1-42 occurred over intracellular and extracellular fibrils that were approximately 8 nm in width. Intracellular beta-amyloid 1-42 fibrils were found in close proximity to glial fibrillary acidic protein fibers within astrocytes, but only in cells with signs of plasma membrane disruption. Neuronal labeling of beta-amyloid 1-42 appears to be associated with the plasma membrane. Membrane-bound beta-amyloid 1-42 occurs in the form of fine fibrils that are embedded in the dendritic membrane and appear to project into the extracellular space as determined by quantitative analysis of the immunogold particle distribution. Bundles of beta-amyloid 1-42 were also closely associated and/or integrated with degenerating myelin sheaths of axons. In one dog that was impaired on several cognitive tasks, extensive beta-amyloid 1-42 deposition was associated with microvacuolar changes and vascular pathology. The present findings suggest that beta-amyloid 1-42 may be generated at the dendritic plasma membrane as well as in intracellular compartments. The close association between beta-amyloid 1-42 and destroyed myelin suggests one possible new mechanism by which beta-amyloid 1-42 induces neurodegeneration.

Published

2000

30. Morphological development of beta(1-40) amyloid fibrils.

Author

Blackley HK, Patel N, Davies MC, Roberts CJ, Tendler SJ, Wilkinson MJ, and Williams PM

Subjects

Amino Acid Sequence, Amyloid beta-Peptides metabolism, Microscopy, Atomic Force, Molecular Sequence Data, Peptide Fragments metabolism, Amyloid beta-Peptides chemistry, Amyloid beta-Peptides ultrastructure, Neurofibrils ultrastructure, Peptide Fragments chemistry, Peptide Fragments ultrastructure

Abstract

The Alzheimer's disease-related peptide beta(1-40) amyloid self-associates to form fibrils exhibiting a morphology characteristic of amyloidogenic proteins. The mechanism of this fibrillization process has yet to be fully elucidated. In this study we have immobilized the beta(1-40) amyloid to flat gold surfaces using thiol-based self-assembled monolayers. Atomic force microscopy reveals the presence of spherical units of beta(1-40) amyloid immediately following the initiation of fibrillization. Short fibrillar structures, termed nascent fibrils, which appear to be formed by the association of these units are also present at this time point. At later time points extended, branching networks of fibrils are observed. Some fibrils exhibit a more beaded appearance and greater axial periodicity than others. No nascent fibrils are seen to be present. We believe that these data identify an early fibril structure which could act as an intermediate in beta-amyloid fibrillization. The oligomeric units of which these nascent fibrils are comprised are also determined., (Copyright 1999 Academic Press.)

Published

1999

31. Taylor's cortical dysplasia: a confocal and ultrastructural immunohistochemical study.

Author

Garbelli R, Munari C, De Biasi S, Vitellaro-Zuccarello L, Galli C, Bramerio M, Mai R, Battaglia G, and Spreafico R

Subjects

Adult, Calbindin 2, Calbindins, Cerebral Cortex metabolism, Cerebral Cortex pathology, Child, Epilepsy etiology, Female, Glial Fibrillary Acidic Protein metabolism, Glutamate Decarboxylase metabolism, Humans, Immunohistochemistry, Intermediate Filaments ultrastructure, Male, Microscopy, Confocal, Microscopy, Electron, Neurofibrils ultrastructure, Neurons metabolism, Neurons pathology, Neurons ultrastructure, Parvalbumins metabolism, Presynaptic Terminals ultrastructure, S100 Calcium Binding Protein G metabolism, Vimentin metabolism, Cerebral Cortex abnormalities, Cerebral Cortex ultrastructure

Abstract

In the present report we describe the neuropathological characteristics of tissue surgically resected from three patients affected by intractable epilepsy secondary to cortical dysplasia. Common features, suggestive of a focal cortical dysplasia of Taylor, were observed in all specimens. Immunocytochemical procedures were performed using neuronal and glial markers and the sections were observed at light traditional and confocal microscopes. This part of the investigation pointed out: 1. cortical laminar disruption; 2. very large neurons displaying a pyramidal or round shape; 3. ballooned cells; 4. decrease of calcium binding proteins immunoreactivity; 5. abnormal nets of parvalbumin- and glutamic acid decarboxylase-positive puncta around giant neurons but not around ballooned cells. Ultrastructural investigation on the same material provided evidence of a high concentration of neurofilaments in giant neurons and of glial intermediate filaments in ballooned cells. In addition, immunolabeled GABAergic terminals clustered around giant neurons were not found to establish synapses on their cell bodies. The present data, derived from a limited sample of patients but showing very consistent features, suggest that in Taylor's type of cortical dysplasia a disturbance of migratory events could be paralleled by a disruption of cell differentiation and maturation and by an impairment of synaptogenesis. This latter mechanism seemed to affect especially the inhibitory elements, and could account for the hyperexcitability of this tissue and thus for the high epileptogenicity of Taylor's dysplasia.

Published

1999

32. A mutation at codon 279 (N279K) in exon 10 of the Tau gene causes a tauopathy with dementia and supranuclear palsy.

Author

Delisle MB, Murrell JR, Richardson R, Trofatter JA, Rascol O, Soulages X, Mohr M, Calvas P, and Ghetti B

Subjects

Adult, Alternative Splicing, Amino Acid Substitution genetics, Brain pathology, Brain ultrastructure, Dementia complications, Dementia pathology, Exons genetics, Humans, Immunohistochemistry, Male, Microscopy, Immunoelectron, Mutation, Neurofibrillary Tangles pathology, Neurofibrils metabolism, Neurofibrils ultrastructure, Neuroglia pathology, Neuroglia ultrastructure, Neurons pathology, Neurons ultrastructure, Parkinson Disease complications, Parkinson Disease genetics, Pedigree, Supranuclear Palsy, Progressive complications, tau Proteins metabolism, Dementia genetics, Supranuclear Palsy, Progressive genetics, tau Proteins genetics

Abstract

Recently intronic and exonic mutations in the Tau gene have been found to be associated with familial neurodegenerative syndromes characterized not only by a predominantly frontotemporal dementia but also by the presence of neurological signs consistent with the dysfunction of multiple subcortical neuronal circuitries. Among families, the symptomatology appears to vary in quality and severity in relation to the specific Tau gene mutation and often may include parkinsonism, supranuclear palsies, and/or myoclonus, in addition to dementia. We carried out molecular genetic and neuropathological studies on two patients from a French family presenting, early in their fifth decade, a cognitive impairment and supranuclear palsy followed by an akinetic rigid syndrome and dementia. The proband died severely demented 7 years after the onset of the symptoms; currently, his brother is still alive although his disease is progressing. In both patients, we found a Tau gene mutation in exon 10 at codon 279, resulting in an asparagine to lysine substitution (N279K). Neuropathologically, widespread neuronal and glial tau accumulation in the cortex, basal ganglia, brain stem nuclei as well as in the white matter were the hallmark of the disease. These deposits were shown by immunohistochemistry and immunoelectron microscopy, using a battery of antibodies to phosphorylation-dependent and phosphorylation-independent epitopes present in multiple tau regions. In the neocortex, tau-immunopositive glial cells were more numerous than immunopositive neurons; the deeper cortical layers as well as the white matter adjacent to the cortex contained the largest amount of immunolabeled glial cells. In contrast, some brain stem nuclei contained more neurons with tau deposits than immunolabeled glial cells. The correlation of clinical, neuropathological and molecular genetic findings emphasize the phenotypic heterogeneity of diseases caused by Tau gene mutations. Furthermore, to test the effect of the N279K mutation and compare it with the effect of the P301L exon 10 mutation on alternative splicing of Tau exon 10, we used an exon amplification assay. Our results suggest that the N279K mutation affects splicing similar to the intronic mutations, allowing exon 10 to be incorporated more frequently in the Tau transcript.

Published

1999

33. Inhibition of fibril formation in beta-amyloid peptide by a novel series of benzofurans.

Author

Howlett DR, Perry AE, Godfrey F, Swatton JE, Jennings KH, Spitzfaden C, Wadsworth H, Wood SJ, and Markwell RE

Subjects

Amyloid beta-Peptides ultrastructure, Antibodies, Benzofurans chemistry, Binding, Competitive, Congo Red metabolism, Drug Evaluation, Preclinical, Formazans, Humans, Hydrogen-Ion Concentration, Immunoassay methods, Inhibitory Concentration 50, Magnetic Resonance Spectroscopy, Microscopy, Electron, Neurofibrils metabolism, Neurofibrils ultrastructure, Peptide Fragments ultrastructure, Protein Binding drug effects, Solubility, Tetrazolium Salts, Time Factors, Amyloid beta-Peptides metabolism, Benzofurans metabolism, Benzofurans pharmacology, Neurofibrils drug effects, Peptide Fragments metabolism

Abstract

A series of benzofuran derivatives have been identified as inhibitors of fibril formation in the beta-amyloid peptide. The activity of these compounds has been assessed by a novel fibril-formation-specific immunoassay and for their effects on the production of a biologically active fibril product. The inhibition afforded by the compounds seems to be associated with their binding to beta-amyloid, as identified by scintillation proximity binding assay. Binding assays and NMR studies also indicate that the inhibition is associated with self-aggregation of the compounds. There is a close correlation between the activity of the benzofurans as inhibitors of fibril formation and their ability to bind to beta-amyloid. Non-benzofuran inhibitors of the fibril formation process do not seem to bind to the same site on the beta-amyloid molecule as the benzofurans. Thus a specific recognition site might exist for benzofurans on beta-amyloid, binding to which seems to interfere with the ability of the peptide to form fibrils.

Published

1999

34. Ultrastructural pathology of a Chilean case of tropical spastic paraparesis/human T-cell lymphotropic type I-associated myelopathy (TSP/HAM).

Author

Liberski PP, Buczyński J, Yanagihara R, Mora C, Gibbs CJ, Gajdusek C, Cartier L, Verdugo A, Araya F, and Castillo L

Subjects

Astrocytes ultrastructure, Axons ultrastructure, Chile, Glycogen metabolism, Humans, Lipofuscin metabolism, Lymphocytes pathology, Myelin Sheath ultrastructure, Myofibrils ultrastructure, Neurofibrils ultrastructure, Vacuoles ultrastructure, Frontal Lobe ultrastructure, Ganglia, Spinal ultrastructure, Muscle, Skeletal ultrastructure, Paraparesis, Tropical Spastic pathology, Spinal Cord ultrastructure

Abstract

Human T-cell lymphotropic virus type I (HTLV-I), is the cause of endemic tropical spastic paraparesis (TSP) or HTLV-I-associated myelopathy (HAM). Because TSP/HAM is not a fatal disease, the neuropathology of this disease, albeit relatively well understood, is based on the examination of just a few incidental cases. Previously, we demonstrated peculiar lamellated structures, called "multilamellar bodies" (MLB). In this report, we present the ultrastructural neuropathology of a TSP/HAM case from Chile, with further detailed descriptions of MLB. It is tempting to suggest that MLB may represent specific ultrastructural markers of TSP/HAM. The pathology of the anterior and posterior horns was similar and was comprised of axonal degeneration, accompanied by extensive astrocytic gliosis. Lymphocytic infiltration, particularly observed as "cuffs" around blood vessels, was scattered among other cellular elements. Ultrastructurally, myelin sheaths were relatively well preserved, and some demyelinated but not remyelinated fibers were observed. Moreover, axons with abnormal accumulations of neurofilaments, suggestive of axonal degeneration, were detected. Several axons contained Hirano bodies. In many samples, glial processes replaced most of the remaining neuropil. In a few specimens of the anterior and posterior horns of the spinal cord, MLB were observed. These structures consisted of stacks of 30 to 40 electron-dense lamellae, which were interrupted by narrow electron-lucent spaces. All of the lamellae were immersed within an amorphous substance of intermediate density. Neurons of the dorsal root ganglia were basically normal except for increased lipofuscin accumulation. As in the spinal cord, myelinated axons were well preserved, but a few were demyelinated and surrounded by concentric arrays of Schwann cell membranes. Also, axons of the dorsal roots accumulated increased number of neurofilaments. Mast cells and Schwann cells were increased in number, the latter containing abundant pi granules and myelin fragments.

Published

1999

35. Basement membranes, microfibrils and beta amyloid fibrillogenesis in Alzheimer's disease: high resolution ultrastructural findings.

Author

Inoue S, Kuroiwa M, and Kisilevsky R

Subjects

Basement Membrane ultrastructure, Humans, Neurofibrils ultrastructure, Alzheimer Disease pathology, Amyloid beta-Peptides physiology, Basement Membrane pathology, Neurofibrils pathology

Abstract

It is known that beta amyloid fibrils are deposited at the basement membrane of the cerebromicrovasculature in the brains of patients with Alzheimer's disease, and the assembly of the fibrils may be in continuation with the core of senile plaques. The fibrils accumulate in a manner similar to that in which microfibrils accumulate in the glomerular basement membrane of the rat kidney during long-term experimental diabetes, and in the alveolar-capillary basement membrane of the normal lung. beta amyloid fibrils in-situ are known to be about 10 nm wide tubular structures and they closely resemble connective tissue microfibrils. Our recent high resolution ultrastructural studies combined with immunogold labeling demonstrated that beta amyloid fibrils in-situ are indeed microfibril-like structures, and the beta protein is associated with their surface in the form of loose assemblies of 1 nm wide flexible filaments. Thus, the result of this study indicates that in-situ a major component of the beta amyloid deposit is the microfibril-like structure. The elucidation of the mechanism of cerebral beta amyloid fibrillogenesis in Alzheimer's disease may therefore require understanding the mechanism of 'normal' microfibrils biogenesis., (Copyright 1999 Elsevier Science B.V.)

Published

1999

36. Astrocytic hyaline inclusions contain advanced glycation endproducts in familial amyotrophic lateral sclerosis with superoxide dismutase 1 gene mutation: immunohistochemical and immunoelectron microscopical analyses.

Author

Kato S, Horiuchi S, Nakashima K, Hirano A, Shibata N, Nakano I, Saito M, Kato M, Asayama K, and Ohama E

Subjects

Adult, Aged, Amyotrophic Lateral Sclerosis genetics, Astrocytes ultrastructure, Cytoplasmic Granules metabolism, Cytoplasmic Granules ultrastructure, Female, Glycation End Products, Advanced immunology, Humans, Immunohistochemistry, Lewy Bodies metabolism, Lewy Bodies ultrastructure, Lysine analogs & derivatives, Lysine metabolism, Male, Microscopy, Immunoelectron, Middle Aged, Mutation, Neurofibrils metabolism, Neurofibrils ultrastructure, Neurons metabolism, Neurons ultrastructure, Superoxide Dismutase metabolism, Superoxide Dismutase-1, Ubiquitins metabolism, Amyotrophic Lateral Sclerosis metabolism, Astrocytes metabolism, Glycation End Products, Advanced metabolism, Hyalin metabolism, Inclusion Bodies metabolism, Superoxide Dismutase genetics

Abstract

To clarify the neuropathological significance of the deposition of N(epsilon)-carboxymethyl lysine (CML), an advanced glycation endproduct, in astrocytic hyaline inclusions in familial amyotrophic lateral sclerosis (FALS), autopsy specimens from five members of two different families who had the superoxide dismutase 1 (SOD1) gene mutations were analysed. Immunohistochemically, most of the neuronal and astrocytic hyaline inclusions were intensely stained by the antibody against CML. The distributions and intensities of the immunoreactivities for CML and SOD1 were similar in the inclusions in both cell types. Immunoelectron microscopy showed that both inclusions consisted of CML-positive granule-coated fibrils and granular materials. No significant CML or SOD1 immunoreactivity was observed in the neurons and astrocytes of the normal control subjects. Our results suggest that astrocytic hyaline inclusions contain CML and SOD1 in FALS patients with SOD1 gene mutations, and that the formation of CML-modified protein (probably CML-modified SOD1) is related to the cell degeneration.

Published

1999

37. Cellular uptake of the prion protein fragment PrP106-126 in vitro.

Author

McHattie SJ, Brown DR, and Bird MM

Subjects

Animals, Cell Count, Cells, Cultured, Cerebellum cytology, Cerebellum metabolism, Immunohistochemistry, Mice, Mice, Inbred C57BL, Microglia chemistry, Microglia ultrastructure, Microscopy, Confocal, Microscopy, Electron, Neurofibrils metabolism, Neurofibrils ultrastructure, Neurons chemistry, Neurons ultrastructure, Peptide Fragments analysis, Peptide Fragments metabolism, Prions analysis, Prions metabolism, Peptide Fragments pharmacokinetics, Prions pharmacokinetics

Abstract

The aetiological agent of prion disease is proposed to be an aberrant isoform of the cell surface glycoprotein known as the prion protein (PrP(c)). This pathological isoform (PrP(Sc)) is abnormally deposited in the extracellular space of diseased CNS. Neurodegeneration in these disease has been shown to be associated with accumulation of PrP(Sc) in affected tissue. To investigate the possible uptake mechanisms that may be required for PrP(Sc)-induced neurodegeneration we studied the cellular trafficking of the neurotoxic fragment, PrP106-126. We were able to detect, by fluorescence microscopy, PrP106-126 inclusions in murine neurones, astrocytes and microglia in vitro. These inclusions were abundant after 24 hour exposure and still present 48h post-exposure. Shorter exposure times yielded only occasional cells with inclusions. Large extracellular aggregates of PrP106-126 could also be detected, which appeared in a time dependent manner. The appearance of inclusions or aggregates was not dependent on PrP(c) expression as determined by exposure of peptides from PrP-null mice. Using transmission electron microscopy and gold particle detection, positively labelled osmiophilic inclusions of peptide could be detected in the cytoplasm of exposed cells. These results demonstrate that cultured cells are capable of sequestering PrP106-126 and may indicate uptake pathways for PrP(Sc) in various cell types. Toxicity of PrP106-126 may thus be mediated via a sequestration pathway that is not effective for this peptide in PrP-null cells.

Published

1999

38. Polyglutamine domain proteins with expanded repeats bind neurofilament, altering the neurofilament network.

Author

Nagai Y, Onodera O, Strittmatter WJ, and Burke JR

Subjects

Amino Acid Sequence, Animals, Cell Line, Green Fluorescent Proteins, Luminescent Proteins genetics, Luminescent Proteins metabolism, Molecular Sequence Data, Neurofibrils ultrastructure, Neurons ultrastructure, Peptides genetics, Recombinant Fusion Proteins metabolism, Repetitive Sequences, Amino Acid, Transfection, Neurofibrils metabolism, Neurofilament Proteins metabolism, Neurons metabolism, Neurons physiology, Peptides metabolism

Abstract

Proteins with expanded polyglutamine (polyQ) repeats cause eight inherited neurodegenerative diseases. Nuclear and cytoplasmic polyQ protein is a common feature of these diseases, but its role in cell death remains debatable. Since the neuronal intermediate filament network is composed of neurofilament (NF) and NF abnormalities occur in neurodegenerative diseases, we examined whether pathologic-length polyQ domain proteins interact with NF. We expressed polyQ-green fluorescent fusion proteins (GFP) in a neuroblast cell line, TR1. Pathologic-length polyQ-GFP fusion proteins form large cytoplasmic aggregates surrounded by neurofilament. Immunoisolation of pathologic-length polyQ proteins co-isolated 68 kD NF protein demonstrating molecular interaction. These observations suggest that polyQ interaction with NF is important in the pathogenesis of the polyglutamine repeat diseases.

Published

1999

39. Fibrilization in mouse senile amyloidosis is fibril conformation-dependent.

Author

Higuchi K, Kogishi K, Wang J, Chen X, Chiba T, Matsushita T, Hoshii Y, Kawano H, Ishihara T, Yokota T, and Hosokawa M

Subjects

Aging, Amyloid metabolism, Amyloid ultrastructure, Animals, Apolipoprotein A-II chemistry, Lipoproteins, HDL blood, Lipoproteins, HDL isolation & purification, Mice, Mice, Mutant Strains, Neurofibrils pathology, Amyloidosis genetics, Amyloidosis pathology, Apolipoprotein A-II genetics, Apolipoprotein A-II metabolism, Liver pathology, Neurofibrils ultrastructure, Spleen pathology

Abstract

Amyloidosis refers to a group of diseases characterized by tissue deposition of amyloid fibrils. A single intravenous injection of a very small amount of the native mouse senile amyloid fibrils (AApoAII) induced severe systemic amyloid deposition in young mice having the amyloidogenic apoA-II gene (Apoa2c). After AApoAII injection, amyloid deposition occurred rapidly and advanced in an accelerated manner, as observed in spontaneous senile amyloidosis in mice. However, the injection of denatured AApoAII, native apoA-II in high-density lipoprotein (HDL), and denatured apoA-II monomer, which have the same primary structure but without a fibril conformation, did not induce amyloidosis. No amyloid deposition was observed in mice having an amyloid-resistant apoA-II gene (Apoa2b) even 3 months after AApoAII injection. Significantly less amyloid deposition was observed in mice having both types of apoA-II genes heterozygously (Apoa2b/c). These findings suggest that the nucleation-dependent polymerization found in vitro also occurs in vivo, and that the fibril conformation is required for the injected amyloid fibrils to act as seeds in vivo. Fibril conformation-dependent fibrillization is proposed as a general model of the pathogenesis of various kinds of amyloidosis occurring in vivo; it may be useful in both elucidating the pathogenesis of amyloidosis and developing effective therapeutic modalities to treat this disease.

Published

1998

40. The N-terminal region of non-A beta component of Alzheimer's disease amyloid is responsible for its tendency to assume beta-sheet and aggregate to form fibrils.

Author

El-Agnaf OM, Bodles AM, Guthrie DJ, Harriott P, and Irvine GB

Subjects

Aging metabolism, Amino Acid Sequence, Amyloid chemistry, Circular Dichroism, Humans, Microscopy, Electron, Molecular Sequence Data, Neurofibrils metabolism, Neurofibrils ultrastructure, Protein Binding, Protein Structure, Secondary, Alzheimer Disease metabolism, Amyloid metabolism

Abstract

Examination of the N-terminal sequence of non-A beta component of Alzheimer's Disease amyloid (NAC) revealed a degree of similarity to regions crucial for aggregation and toxicity of three other amyloidogenic proteins, namely amyloid beta peptide (A beta), prion protein (PrP) and islet amyloid polypeptide (IAPP), leading us to believe that this might be the part of the molecule responsible for causing aggregation. Secondary structure prediction analysis of NAC indicated that the N-terminal half was likely to form a beta-structure whereas the C-terminal half was likely to form an alpha-helix. NAC in solution altered from random coil to beta-sheet structure upon ageing, a process that has previously been shown to lead to fibril formation. To delineate the region of NAC responsible for aggregation we synthesised two fragments, NAC-(1-18)-peptide and NAC-(19-35)-peptide, and examined their physicochemical properties. Upon incubation, solutions of NAC-(1-18)-peptide became congophilic and aggregated to form fibrils of diameter 5-10 nm, whereas NAC-(19-35)-peptide did not bind Congo Red and remained in solution. Circular dichroism spectroscopy was used to study the secondary structure of NAC and the two fragments. In trifluoroethanol/water mixtures, NAC and NAC-(19-35)-peptide adopted alpha-helical structure but NAC-(1-18)-peptide did not. NAC-(1-18)-peptide and NAC formed beta-sheet in acetonitrile/water mixtures more readily than did NAC-(19-35)-peptide. CD spectra of NAC or NAC-(1-18)-peptide in aqueous solution indicate the formation of beta-sheet on ageing. We propose that the N-terminal region of NAC is the principal determinant of aggregation. Our results indicate that NAC resembles A beta, and other amyloidogenic proteins, in that aggregation is dependent upon beta-sheet development. These results lend support to a role for NAC in the development of neurodegenerative disease.

Published

1998

41. Immunohistochemical and ultrastructural characterization of ubiquitinated eosinophilic fibrillary neuronal inclusions in sporadic amyotrophic lateral sclerosis.

Author

Arima K, Ogawa M, Sunohara N, Nishio T, Shimomura Y, Hirai S, and Eto K

Subjects

Amyotrophic Lateral Sclerosis metabolism, Autopsy, Brain pathology, Brain Chemistry physiology, Crystallins metabolism, Eosinophils pathology, Eosinophils ultrastructure, Humans, Immunohistochemistry, Inclusion Bodies metabolism, Male, Microscopy, Immunoelectron, Middle Aged, Neurofibrillary Tangles pathology, Neurofibrils metabolism, Neurons metabolism, Amyotrophic Lateral Sclerosis pathology, Inclusion Bodies pathology, Inclusion Bodies ultrastructure, Neurofibrils pathology, Neurofibrils ultrastructure, Neurons pathology, Neurons ultrastructure, Ubiquitins metabolism

Abstract

We found eosinophilic fibrillary neuronal inclusions (EFNI) that were argyrophilic and immunoreactive for anti-ubiquitin in the cerebral cortex of a patient with sporadic amyotrophic lateral sclerosis (ALS) and mild personality changes. Both hematoxylin and eosin and Bodian's preparations revealed the EFNI to be rod-, flame-shaped, or spherical structures existing within the swollen neuronal perinuclear region in the third, fifth, and sixth layers of the fronto-parieto-temporal cortices including the primary motor cortex. On electron microscopy, filamentous profiles aggregated and formed a single bundle or globule in the neuronal perikaryon without any limiting membrane. Most EFNI had a characteristic multiple layer arrangement. The inner core consisted of randomly oriented granule-free tubules with a fuzzy outer contour, measuring 15-20 nm in diameter. The surrounding layer was made up of granule-associated filaments, electrondense free granules, and small vesicular profiles. Large autolysosome-like membrane-bound vesicular profiles were found scattered at the periphery. Neurofilaments were usually mingled with in the surrounding cytoplasm. Many EFNI were also found in dendrites, but only a few in axons. Both granule-free tubules and granule-associated filaments expressed ubiquitin protein epitopes. Aberrant phosphorylation of neurofilament protein and induction of alphaB-crystallin were shown to exist in EFNI-bearing swollen neurons. Despite having a variety of histological appearances, our observations revealed that EFNI all have common immunocytochemical and ultrastructural characteristics, and thus we assume that EFNI represent a series of cytological alterations in the motor and extra-motor cortices of ALS patients.

Published

1998

42. The distribution of scrapie-associated fibrils in neural and non-neural tissues of advanced clinical cases of natural scrapie in sheep.

Author

Stack MJ, Chaplin MJ, Aldrich AM, and Davis LA

Subjects

Animals, Intestines pathology, Lymph Nodes pathology, Microscopy, Electron, Neurofibrils ultrastructure, Organ Specificity, Palatine Tonsil pathology, Pituitary Gland pathology, Sciatic Nerve pathology, Sheep, Spinal Cord pathology, Spleen pathology, Brain pathology, Neurofibrils pathology, Scrapie pathology

Abstract

The distribution of scrapie-associated fibrils (SAFs) throughout four brain regions, the pituitary gland, along the whole length of the spinal cord and in the sciatic nerve was assessed in 10 sheep terminally affected by scrapie and in four control sheep. Tonsils, retropharyngeal, broncho-mediastinal and mesenteric lymph nodes, the distal ileum, proximal colon and spleen were also examined for fibrils in all 14 sheep. Fibrils were detected in all four brain regions and throughout the length of the spinal cord in nine of the scrapie affected sheep. SAFs were not detectable in any of the sciatic nerve samples tested. In one of the 10 clinically affected sheep only minimal lesions were found by histopathology and fibrils were detected only from the cerebrum and one spinal cord region (taken at the C1 C2 vertebrae). Fibrils were not detected in the tonsils or retropharyngeal lymph nodes but were detected in other non-neural tissues of some of the scrapie-affected sheep. These tissues included pituitary gland, broncho-mediastinal and mesenteric portal lymph nodes, distal ileum, proximal colon and spleen. Fibrils could not be detected in any of the tissues taken from the four control sheep.

Published

1998

43. Cognitive, neuroimaging, and pathological studies in a patient with Pick's disease.

Author

Lieberman AP, Trojanowski JQ, Lee VM, Balin BJ, Ding XS, Greenberg J, Morrison D, Reivich M, and Grossman M

Subjects

Aged, Amygdala pathology, Atrophy, Cerebrovascular Circulation, Cognition Disorders diagnosis, Dementia physiopathology, Dentate Gyrus pathology, Fatal Outcome, Hippocampus pathology, Humans, Magnetic Resonance Imaging, Male, Microscopy, Electron, Neurofibrils ultrastructure, Neurons pathology, Tomography, Emission-Computed, tau Proteins analysis, Cerebral Cortex pathology, Dementia diagnosis

Abstract

We conducted cognitive, imaging, and neuropathological studies on a patient with Pick's disease. The patient was impaired at interpreting sentences with complex grammatical constructions, differing significantly from control subjects and patients with Alzheimer's disease (AD). Evaluation of regional brain functioning at rest, with positron emission tomography, revealed reduced left frontal activity compared with control subjects and AD patients. Autopsy demonstrated the classic pathology of Pick's disease, including massive neuron loss and gliosis in the frontal and cingulate cortex as well as numerous tau-positive hippocampal Pick bodies. The abnormal tau proteins were phosphorylated at the same amino acid residues as AD paired helical filament tau (PHFtau), but they exhibited a unique migration profile on western blot. Our observations support the hypothesis that a distinct variety of hyperphosphorylated tau in Pick's disease compromises the long-term viability of selectively vulnerable populations of neurons in frontal cortices that contribute to sentence processing.

Published

1998

44. Amidation of beta-amyloid peptide strongly reduced the amyloidogenic activity without alteration of the neurotoxicity.

Author

Forloni G, Lucca E, Angeretti N, Della Torre P, and Salmona M

Subjects

Amino Acid Sequence, Amyloid beta-Peptides chemistry, Animals, Apoptosis drug effects, Cell Nucleus drug effects, Cell Nucleus pathology, Cell Nucleus ultrastructure, Cell Survival drug effects, Cells, Cultured, Culture Media, DNA Fragmentation, Fetus, Hippocampus cytology, Microscopy, Electron, Neurofibrils drug effects, Neurofibrils pathology, Neurofibrils ultrastructure, Neurons pathology, Peptide Fragments chemistry, Peptides chemical synthesis, Peptides chemistry, Peptides toxicity, Rats, Amyloid beta-Peptides toxicity, Hippocampus pathology, Neurons drug effects, Neurotoxins, Peptide Fragments toxicity

Abstract

Beta-amyloid accumulates in cerebral deposits in Alzheimer's disease, so to test the correlation between the neurotoxic and fibrillogenic capacity of beta-amyloid, we synthesized a peptide homologous to fragment 25-35 of beta-amyloid (beta25-35) and amidated at the C-terminus (beta25-35-NH2). As the amidation strongly reduced the amyloidogenic capacity of beta25-35, we compared its neurotoxic activity in the amidated (beta25-35-NH2) and nonamidated forms. The viability of primary cultures from fetal rat hippocampus was reduced in a dose-related manner (10-100 microM) similarly by beta25-35 and beta25-35-NH2, whereas a scrambled peptide, amidated or nonamidated, did not alter the neuronal viability. The neurotoxic activity of beta25-35-NH2 is mediated by apoptosis as demonstrated by morphological and biochemical investigations. Electron microscopy examination of culture media with beta25-35 or beta25-35-NH2 incubated with neuronal cells for 7 days confirmed the high level of fibrillogenic activity of beta25-35 and the almost total absence of fibrils in the solution with beta25-35-NH2. Furthermore, staining with thioflavine S was used to identify amyloid fibrils, and only the cultures exposed to beta25-35 exhibited intense staining associated with neuronal membranes. These data indicate that the neurotoxic activity of the beta-amyloid fragment is independent of the aggregated state of the peptide.

Published

1997

45. Neurofilaments are part of the high molecular weight complex containing neuronal cdc2-like kinase (nclk).

Author

Lee KY and Johnston RN

Subjects

Animals, Brain cytology, Brain enzymology, Cattle, Chromatography, Gel, Cyclin-Dependent Kinase 5, Electrophoresis, Polyacrylamide Gel, Molecular Weight, Neurofibrils ultrastructure, Cyclin-Dependent Kinases, Neurofibrils enzymology, Neurofilament Proteins analysis, Protein Serine-Threonine Kinases analysis

Abstract

A cdc2-like kinase (nclk, comprised of cdk5 and its activator p25nck5a) that localizes primarily to neuronal cells has recently been identified. Although its precise physiological role remains unclear, a variety of nuclear and cytoplasmic proteins that may be targets for phosphorylation by this kinase have been suggested in various developmental and pathological states. Here we provide evidence for a functional association between nclk and neurofilament proteins: (i) brain neurofilament preparations include cdk5 and p25nck5a; (ii) nclk copurifies with neurofilament proteins using Mono-S and gel-filtration column chromatographic procedures; (iii) neurofilaments are coprecipitated with cdk5 kinase; and (iv) the addition of radiolabeled ATP to the immunoprecipitated complex results in phosphorylation of the cytoskeletal protein. These results are consistent with the formation of a functional macromolecular complex between nclk and neurofilaments in vivo and suggest a possible role for this kinase in regulating neuronal cytoskeletal networks.

Published

1997

46. Paired helical filaments in corticobasal degeneration: the fine fibrillary structure with NanoVan.

Author

Tracz E, Dickson DW, Hainfeld JF, and Ksiezak-Reding H

Subjects

Aged, Aged, 80 and over, Aurothioglucose, Brain ultrastructure, Coloring Agents, Female, Humans, Male, Microscopy, Electron, Neurofibrils ultrastructure, Organometallic Compounds, Vanadates, tau Proteins analysis, Alzheimer Disease pathology, Brain pathology, Neurodegenerative Diseases pathology, Neurofibrils pathology

Abstract

Paired helical filaments (PHF) composed of hyperphosphorylated tau proteins are characteristic findings in neurodegenerative disorders, including Alzheimer's disease (AD) and corticobasal degeneration (CBD). The filaments in CBD differ from those in AD by a reduced number of tau isoforms and less stable ultrastructure. To further compare the ultrastructure of both filaments, we employed a novel staining reagent, NanoVan, as well as aurothioglucose and uranyl acetate. With commonly used uranyl acetate, both kinds of filaments appeared as twisted ribbons 15-20-nm and 21-23-nm wide, respectively, without significant internal substructure. With application of aurothioglucose, only few structural details were apparent. With NanoVan, AD filaments showed similar structure to that with uranyl acetate but CBD filaments displayed a highly heterogeneous appearance consistent with the dissociation of the 20-25-nm-wide filaments along two longitudinal axes. This was evident by the presence of thinner, 12-13-nm-wide filaments and filaments that splayed into two 20-25-nm-wide components at one or both ends. Moreover, detection of a prominent, 7-8-nm-wide axial region distinguished up to four protofilaments per one filament. Each protofilament appeared to contain two 3-5-nm-wide fibrils separated by an approximately 1-nm-wide axial region. The results suggest that 3-5-nm fibrils are the smallest structural subunits of filaments in CBD and that NanoVan may be an unique reagent in detecting eight-fibril organization in these less stable filaments.

Published

1997

47. Loss of axonal microtubules and neurofilaments after stretch-injury to guinea pig optic nerve fibers.

Author

Maxwell WL and Graham DI

Subjects

Analysis of Variance, Animals, Case-Control Studies, Cross-Sectional Studies, Guinea Pigs, Microscopy, Electron, Optic Nerve ultrastructure, Ranvier's Nodes ultrastructure, Stress, Mechanical, Time Factors, Axons ultrastructure, Disease Models, Animal, Microtubules ultrastructure, Neurofibrils ultrastructure, Optic Nerve Injuries

Abstract

Axonal swellings, characterized by focal accumulations of membranous organelles at presumed sites of interrupted axonal transport, occur in diffuse axonal injury (DAI) in human, blunt head injury and in animal models of nondisruptive axonal injury. Membranous organelles are transported by fast axonal transport in association with microtubules. Although loss of microtubules has been documented at levels of injury severe enough to result in permeabilization of the axolemma to tracers such as horseradish peroxidase, there has been no detailed analysis of responses by microtubules in less severe or milder forms of nondisruptive axonal injury. To test the hypothesis that in less severe forms of axonal injury there is a rapid response by axonal microtubules that might provide an explanation for loss of fast axonal transport, we have carried out a morphometric analysis of microtubules in CNS axons after stretch-injury. There is loss of microtubules at nodes of Ranvier with nodal blebs within 15 min of injury, and in internodal axonal swellings between 2 and 4 h. There is a return to control values at nodes of Ranvier by 4 h, and at the internode by 24 h. There is no loss of microtubules at paranodes, although there is a reduction in their density in the first 2 h after injury. The greatest loss of microtubules occurs at sites of axolemma infolding. Hypothetical mechanisms that might lead to this loss resulting in focal disruption of fast axonal transport and the formation of axonal swellings are discussed.

Published

1997

48. Investigation of effect of lesser curvature seromyotomy of the stomach in animal experiments.

Author

Bátorfi J, Kovács V, Bajtai A, Hidvegi J, Dabasi G, Pósfai G, Tóth J, and Ihász M

Subjects

Animals, Dogs, Electrodes, Female, Gastric Acid metabolism, Gastric Emptying, Hydrogen-Ion Concentration, Male, Neurofibrils ultrastructure, Stomach physiology, Stomach ultrastructure, Stomach innervation, Vagotomy, Proximal Gastric methods

Abstract

The effectiveness of seromyotomy of the lesser curvature of the stomach--the simplified version of proximal selective vagotomy--was investigated in eleven dogs. Decreased acid secretion was proved with congo red test and pH measuring by glass electrode. No significant damage to the motor function of the stomach was found with scintigraphy. Histological examinations revealed neurofibre degeneration peripherally to the seromyotomy line after peripheral vagotomy and vacuolar degeneration in the ganglion cells and amputation neuromas in the seromyotomy line.

Published

1997

49. Comparison of detergent and protease enzyme combinations for the detection of scrapie-associated fibrils from the central nervous system of sheep naturally affected with scrapie.

Author

Stack MJ, Aldrich AM, and Davis LA

Subjects

Animals, Drug Combinations, Female, Microscopy, Electron, Sheep, Central Nervous System pathology, Detergents, Endopeptidases, Neurofibrils ultrastructure, Scrapie pathology, Sheep Diseases pathology

Abstract

Standardized samples of tissue from the central nervous system of four sheep naturally affected with scrapie and from four healthy control sheep were subjected to a centrifugal extraction technique used to obtain scrapie-associated fibrils; the latter were then demonstrated by negative-contrast transmission electron microscopy. This regime was used to evaluate the fibril yield obtained from the 25 possible combinations of five different detergents and five different proteolytic enzymes. N-lauroylsarcosine detergent was found to be the most efficient detergent for all five enzymes, followed by sulphabetaine 3-14. Sodium dodecyl sulphate detergent was successful only in combination with a subtilisin Carlsberg enzyme. Octylglucoside and nonidet P40 detergents did not produce fibrils with any of the enzymes. Proteinase K was the least efficient of the five enzymes when used in combination with N-lauroylsarcosine; subtilisin Carlsberg, clostripain, pronase and trypsin enzymes all gave higher fibril yields. A combination of N-lauroylsarcosine detergent and subtilisin Carlsberg proteolytic enzyme gave the highest fibril yield.

Published

1997

50. Distribution of amyloid beta-protein immunoreactivity in the hippocampus of rats injected with kainate.

Author

Ong WY, He Y, and Garey LJ

Subjects

Amyloid beta-Peptides analysis, Animals, Astrocytes pathology, Astrocytes ultrastructure, Hippocampus drug effects, Hippocampus pathology, Immunohistochemistry, Male, Microscopy, Immunoelectron, Mitochondria metabolism, Mitochondria ultrastructure, Neurofibrils metabolism, Neurofibrils ultrastructure, Neuropil metabolism, Neuropil ultrastructure, Rats, Rats, Wistar, Time Factors, Amyloid beta-Peptides biosynthesis, Astrocytes metabolism, Excitatory Amino Acid Agonists toxicity, Hippocampus metabolism, Kainic Acid toxicity

Abstract

The distribution of amyloid beta-protein immunoreactivity was investigated in the hippocampus of rats injected intravenously with kainate. Very light labelling was observed in cell bodies and dendrites of pyramidal neurons and dentate granule cells in the normal hippocampus. At 6,7,9,10,12 and 20 days postinjection, moderately densely labelled astrocytes were present in the stratum oriens and lacunosum moleculare, extending thick processes towards the stratum radiatum which was degenerating. Immunoreactivity was present as floccules in the mitochondria-rich but glial-filament-poor portions of reactive astrocytes, and in fibrillar form in the neuropil. This suggests that amyloid beta-protein might be present in fibrillar (presumably polymerised) form in degenerating profiles and the neuropil, but in floccular (presumably non-polymerised) form in reactive astrocytes.

Published

1997