User:Alexanae/Chromatolysis Draft

History[edit]

In 1885, researcher W. Flemming described dying cells in degenerating mammalian ovarian follicles. The cells showed variable stages of pyknotic chromatin. These stages included chromatin condensation, which Flemming described as “half-moon” shaped and appearing as “chromatin balls” (large, smooth, and round electron-dense chromatin masses). Other stages included cell fractionation into smaller bodies. Flemming named this degenerative process “chromatolysis” to describe the gradual disintegration of nuclear components. The process he described now fits with the relatively new term, apoptosis, to describe cell death.

Around the same time of Flemming’s research, chromatolysis was also studied in the lactating mammary glands and in breast cancer cells. Based on the findings of these studies, some researchers argued for the existence of a necessary cellular process to counterbalance the proliferation of cells by mitosis. It was proposed that chromatolysis played a major role in this physiological process. Chromatolysis was also thought to be responsible for necessary cell elimination in various organs during development. Again, these expanded definitions of chromatolysis are consistent with what we now term apoptosis.

In 1952, research further supported the role of chromatolysis in changing the physiology of cells during cell death processes in embryo development. It was also observed that the integrity of mitochondria is maintained during chromatolysis.

By the 1970s, studies identified the conserved structural features of chromatolysis. The consistent features of chromatolysis included the condensation of the cytoplasm and chromatin, cell shrinkage, formation of “chromatin balls,” intact normal organelles, and fragmentation of cells observed by the budding of fragments enclosed in the cell membrane. These budding fragments were termed “apoptotic bodies,” thus coining the name “apoptosis” to describe this form of cell death. The authors of these studies, most likely unfamiliar with older publications on chromatolysis, were essentially describing a process identical to chromatolysis.^[1]

Types of Chromatolysis[edit]

Central Chromatolysis[edit]

Central chromatolysis is the most common form of chromatolysis and is characterized by the loss or dispersion of the Nissl bodies starting in the center of the neuron (around the nucleus) and then extending peripherally towards the plasma membrane.

Peripheral Chromatolysis[edit]

Peripheral chromatolysis is much less common, but has been reported to occur after axotomy and ischemia in certain species. Peripheral chromatolysis is essentially the reverse of central chromatolysis, in which the disintegration of Nissl bodies is initiated at the periphery of the neuron and extends inwards towards the nucleus of the cell. Peripheral chromatolysis has been observed to occur in lithium-induced chromatolysis and it could be useful in investigating and countering the hypothesis that waves of enzymatic activity always progress from the perinuclear area to the peripheral of the cell.^[2]

Causes[edit]

Nissl Bodies[edit]

Studies have shown that injury to spinal motor neurons results in increased size of the nucleolus, nucleus, and cell body. The nucleus becomes elongated and organization of Nissl bodies is disrupted. The process of Nissl dissolution is less apparent toward periphery of the cell body of the neuron, where normal-looking Nissl bodies may be present.^[3] This loss of Nissl bodies propagating from the center of the cell body outward is known as central chromatolysis. In neurons receiving axonal transection, central chromatolysis is observed in the area between the nucleus and the axon hillock following.

The enlargement of nuclear components due to axotomy can be explained by the alteration of the cell’s cytoskeleton. The cytoskeleton maintains the nuclear components of a cell and the size of the cell body in neurons. The increase in protein within the neuron leads to this change in the cytoskeleton. The increase in protein can be explained by the increase in cytoskeleton size. Changes in the cell body cytoskeleton seem to be responsible for enhanced nuclear eccentricity following axonal injury.

One hypothesis behind the incidence of chromatolysis following axotomy is that the shortening of the axon prevents the incorporation of the axonal cytoskeleton that undergoes formation in the injured neuron. Nuclear eccentricity can be attributed to the presence of excess axonal cytoskeleton between the nucleus and axon hillock, which causes chromatolysis. A second hypothesis proposes that blockage of axonal cytoskeletal proteins causes chromatolysis.

Central chromatolysis is the loss of basophilic staining after axotomy. The loss of staining begins near the nucleus and spreads toward the axon hillock. The basophilic rim is formed as chromatolysis compresses the cytoplasmic skeleton.^[4]

Acrylamide Intoxication[edit]

Acrylamide intoxication has been shown to be an agent for the induction of chromatolysis. In one study groups of rats were injected with acrylamide for 3, 6, and 12 days and the A- and B-cell perikarya of their L5 dorsal root ganglion were examined. There was no morphological change in the B-cell perikarya, the A-cell perikarya however exhibited chromatolysis in 11% and 23% of the population, for the 6 and 12 days groups respectively. Acrylamide intoxication resembles neural axotomy histologically and mechanically. In each case the neuron undergoes chromatolysis and atrophy of the cell body and axon. Also both seem to be mechanically related to a disruption of the delivery of neurofilament to the axon due to a decreased transport of a trophic factor from the axon to the cell body.^[5]

Associated Diseases[edit]

Amyotrophic Lateral Sclerosis (ALS)[edit]

Central chromatolysis has been observed in anterior horn neurons of patients with amyotrophic lateral sclerosis (ALS). Patients with ALS appear to have significant alterations that occur within the chromatolyzed neuronal cells. These alterations include dense conglomerates of aggregated dark mitochondria and presynaptic vesicles, bundles of neurofilaments, and a marked increase of presynaptic vesicles. Changes to the function of the motor neurons have also been observed. The most typical functional change in chromatolytic motor neurons is the significant reduction in size of the monosynaptic excitatory postsynaptic potentials (EPSPs). These monosynaptic EPSPs also seem to be prolonged in the chromatolyzed cells of ALS patients. This functional change to the anterior horn neurons could result in the elimination of certain excitatory synaptic inputs and thus give rise to the clinical motor function impairment that is characteristic of the ALS disease. ^[6]

Idiopathic Brainstem Neuronal Chromatolysis[edit]

Severe neuronal chromatolysis has been detected in the brainstems of adult cattle with the neurodegenerative condition known as idiopathic brainstem neuronal chromatolysis (IBNC). The disease has a significant correlation with abnormal labeling for prion protein (PrP) in the brain. IBNC has also been characterized by severe neuronal, axonal, and myelin degradation, accompanied by non-supportive inflammation and changes in spongiform of various regions of grey matter. A significant loss of neurons due to hippocampal degeneration has also been observed. The degenerate chromatolysis neurons seldom showed intracytoplasmic labeling for PrP.^[7]

References[edit]

^ Stoica, Bogdan; Faden, Alan (2010). "Programmed Neuronal Cell Death Mechanisms in CNS Injury". Acute Neuronal Injury. 4: 169–200. doi:10.1007/978-0-387-73226-8_12.
^ Levine, Seymour; Saltzman, Arthur; Kumar, Asok R (2004). "A Method for Peripheral Chromatolysis in Neurons of Trigeminal and Dorsal Root Ganglia, Produced in Rats by Lithium". Journal of Neuroscience Methods. 132: 1–7. PMID 14687669.
^ Gersh, I.; IBodian, D. (1943). "Some chemical mechanisms in chromatolysis". Journal of Cellular and Comparative Physiology. 21: 253–279. doi:10.1002/jcp.1030210305.
^ McIlwain, David; Hoke, Victoria (2005). "The role of the cytoskeleton in cell body enlargement, increased nuclear eccentricity and chromatolysis in axotomized spinal motor neurons". BMC Neuroscience. 6: 16. PMC 1079867. PMID 15774011.
^ Tandrup, T. (2002). "Chromatolysis of A-cells of dorsal root ganglia is a primary structural event in acute acrylamide intoxication". Journal of Neurocytology. 31: 73–78. {{cite journal}}: line feed character in |title= at position 87 (help)
^ Sasaki, Shoichi; Iwata, Makoto (1996). "Ultrastructural study of synapses in the anterior horn neurons of patients with amyotrophic lateral sclerosis". Neuroscience Letters. 204: 53–56. PMID 8929976.
^ Jeffrey, Martin; Perez, Belinda; Terry, Linda; González, Lorenzo (2008). "Idiopathic Brainstem Neuronal Chromatolysis (IBNC): a novel prion protein related disorder of cattle?". BMC Veterinary Research. 4: 1–38. doi:10.1186/1746-6148-4-38.{{cite journal}}: CS1 maint: unflagged free DOI (link)

[“Stoica”-1] Stoica, Bogdan; Faden, Alan (2010). "Programmed Neuronal Cell Death Mechanisms in CNS Injury". Acute Neuronal Injury. 4: 169–200. doi:10.1007/978-0-387-73226-8_12.

[“levine”-2] Levine, Seymour; Saltzman, Arthur; Kumar, Asok R (2004). "A Method for Peripheral Chromatolysis in Neurons of Trigeminal and Dorsal Root Ganglia, Produced in Rats by Lithium". Journal of Neuroscience Methods. 132: 1–7. PMID 14687669.

[“Gersh”-3] Gersh, I.; IBodian, D. (1943). "Some chemical mechanisms in chromatolysis". Journal of Cellular and Comparative Physiology. 21: 253–279. doi:10.1002/jcp.1030210305.

[“mcilwain”-4] McIlwain, David; Hoke, Victoria (2005). "The role of the cytoskeleton in cell body enlargement, increased nuclear eccentricity and chromatolysis in axotomized spinal motor neurons". BMC Neuroscience. 6: 16. PMC 1079867. PMID 15774011.

[“tandrup”-5] Tandrup, T. (2002). "Chromatolysis of A-cells of dorsal root ganglia is a primary structural event in acute acrylamide intoxication". Journal of Neurocytology. 31: 73–78. {{cite journal}}: line feed character in |title= at position 87 (help)

[“Sasaki”-6] Sasaki, Shoichi; Iwata, Makoto (1996). "Ultrastructural study of synapses in the anterior horn neurons of patients with amyotrophic lateral sclerosis". Neuroscience Letters. 204: 53–56. PMID 8929976.

[“Jeffrey”-7] Jeffrey, Martin; Perez, Belinda; Terry, Linda; González, Lorenzo (2008). "Idiopathic Brainstem Neuronal Chromatolysis (IBNC): a novel prion protein related disorder of cattle?". BMC Veterinary Research. 4: 1–38. doi:10.1186/1746-6148-4-38.{{cite journal}}: CS1 maint: unflagged free DOI (link)

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