Inclusion bodies
Inclusion bodies, sometimes called elementary bodies, are nuclear or cytoplasmic aggregates of stable substances, usually proteins. They typically represent sites of viral multiplication in a bacterium or a eukaryotic cell and usually consist of viral capsid proteins. Inclusion bodies can also be hallmarks of genetic diseases, as in the case of neuronal inclusion bodies in disorders like frontotemporal dementia and Parkinson's disease.[1]
Inclusion bodies contain very little host protein, ribosomal components or DNA/RNA fragments. They often almost exclusively contain the over expressed protein and aggregation in inclusion bodies has been reported to be reversible. It has been suggested that inclusion bodies are dynamic structures formed by an unbalanced equilibrium between aggregated and soluble proteins of Escherichia coli. There is a growing body of information indicating that formation of inclusion bodies occurs as a result of intracellular accumulation of partially folded expressed proteins which aggregate through non-covalent hydrophobic or ionic interactions or a combination of both.
Inclusion bodies are dense electron-refractile particles of aggregated protein found in both the cytoplasmic and periplasmic spaces of E. coli during high-level expression of heterologous protein. It is generally assumed that high level expression of non-native protein (higher than 2% of cellular protein) and highly hydrophobic protein is more prone to lead to accumulation as inclusion bodies in E. coli.[citation needed] In the case of proteins having disulfide bonds, formation of protein aggregates as inclusion bodies is anticipated since the reducing environment of bacterial cytosol inhibits the formation of disulfide bonds. The diameter of spherical bacterial inclusion bodies varies from 0.5–1.3 μm and the protein aggregates have either an amorphous or paracrystalline nature depending on the localization.[citation needed] Inclusion bodies have higher density (~1.3 mg ml−1) than many of the cellular components, and thus can be easily separated by high-speed centrifugation after cell disruption. Inclusion bodies despite being dense particles are highly hydrated and have a porous architecture.[2]
Composition
Inclusion bodies have a non-unit lipid membrane. Protein inclusion bodies are classically thought to contain misfolded protein. However, this has recently been contested, as green fluorescent protein will sometimes fluoresce in inclusion bodies, which indicates some resemblance of the native structure and researchers have recovered folded protein from inclusion bodies.[3][4][5]
Mechanism of formation
When genes from one organism are expressed in another organism the resulting protein sometimes forms inclusion bodies. This is often true when large evolutionary distances are crossed: a cDNA isolated from Eukarya for example, and expressed as a recombinant gene in a prokaryote risks the formation of the inactive aggregates of protein known as inclusion bodies. While the cDNA may properly code for a translatable mRNA, the protein that results will emerge in a foreign microenvironment. This often has fatal effects, especially if the intent of cloning is to produce a biologically active protein. For example, eukaryotic systems for carbohydrate modification and membrane transport are not found in prokaryotes. The internal microenvironment of a prokaryotic cell (pH, osmolarity) may differ from that of the original source of the gene. Mechanisms for folding a protein may also be absent, and hydrophobic residues that normally would remain buried may be exposed and available for interaction with similar exposed sites on other ectopic proteins. Processing systems for the cleavage and removal of internal peptides would also be absent in bacteria. The initial attempts to clone insulin in a bacterium suffered all of these deficits. In addition, the fine controls that may keep the concentration of a protein low will also be missing in a prokaryotic cell, and overexpression can result in filling a cell with ectopic protein that, even if it were properly folded, would precipitate by saturating its environment.[citation needed]
Viral inclusion bodies
Examples of viral inclusion bodies in animals are
Intracytoplasmic eosinophilic (acidophilic)-
- Negri bodies in Rabies
- Guarnieri bodies in vaccinia, variola (smallpox)
- Paschen bodies in variola (smallpox)
- Bollinger bodies in fowlpox
- Henderson-Patterson bodies in Molluscum contagiosum
- Eosinophilic inclusion bodies in boid inclusion body disease
Intranuclear eosinophilic (acidophilic)-
- Cowdry type A in Herpes simplex virus and Varicella zoster virus
- Torres bodies in Yellow fever
- Cowdry type B in Polio and adenovirus
Intranuclear basophilic-
- Cowdry type B in Adenovirus
- "Owl's eye appearance" in cytomegalovirus
Both intranuclear and intracytoplasmic-
Examples of viral inclusion bodies in plants[6] include aggregations of virus particles (like those for Cucumber mosaic virus[7]) and aggregations of viral proteins (like the cylindrical inclusions of potyviruses[8]). Depending on the plant and the plant virus family these inclusions can be found in epidermal cells, mesophyll cells, and stomatal cells when plant tissue is properly stained.[9]
Inclusion bodies in Erythrocytes
Normally a red blood cell does not contain inclusions in the cytoplasm. However, it may be seen because of certain hematologic disorders.
There are three kinds of erythrocyte inclusions:
- Developmental Organelles
- Howell-Jolly bodies: small, round fragments of the nucleus resulting from karyorrhexis or nuclear disintegration of the late reticulocyte and stain reddish-blue with Wright stain.
- Basophilic stipplings - these stipplings are either fine or coarse, deep blue to purple staining inclusion that appears in erythrocytes on a dried Wright stain.
- Pappenheimer bodies - are siderotic granules which are small, irregular, dark-staining granules that appear near the periphery of a young erythrocyte in a Wright stain.
- Polychromatophilic red cells - young red cells that no longer have nucleus but still contain some RNA.
- Cabot Rings - ring-like structure and may appear in erythrocytes in megaloblastic anemia or in severe anemias, lead poisoning, and in dyserythropoiesis, in which erythrocytes are destroyed before being released from the bone marrow.
- Abnormal Hemoglobin Precipitation
- Heinz bodies - round bodies, refractile inclusions not visible on a Wright stain film. It is best identified by supravital staining with basic dyes.
- Hemoglobin H Inclusions - alpha thalassemia, greenish-blue inclusion bodies appear in many erythrocytes after four drops of blood is incubated with 0.5mL of Brilliant cresyl blue for 20 minutes at 37 °C.
- Protozoan Inclusion
Inclusion bodies in Bacteria
Polyhydroxyalkanoates or PHA are produced by bacteria as inclusion bodies, the size of PHA granules are limited in E. coli, due to its small bacterial size.[10] Bacterial cell's inclusion bodies are not as abundant intracellularly, in comparison to eukaryotic cells.
Current problems with the isolation of proteins from bacterial inclusion bodies
70-80% of recombinant proteins expressed E. coli are contained in inclusion bodies (i.e., protein aggregates).[11] The purification of the expressed proteins from inclusion bodies usually require two main steps: extraction of inclusion bodies from the bacteria followed by the solubilisation of the purified inclusion bodies. Solubilisation of inclusions bodies often involves treatment with denaturing agents, such as urea or guanidine chloride at high concentrations, to de-aggregate the collapsed proteins. Renaturation follows the treatment with denaturing agents and often consists of dialysis and/or use of molecules that promote the refolding of denatured proteins (including chaotopic agents[12] and chaperones).[13]
Pseudo-inclusions
Pseudo-inclusions are invaginations of the cytoplasm into the cell nuclei, which may give the appearance of intranuclear inclusions. They may appear in papillary thyroid carcinoma.[14]
Diseases involving inclusion bodies
Disease | Affected cells |
---|---|
Inclusion body myositis | muscle cells |
Amyotrophic lateral sclerosis | motor neurons |
Dementia with Lewy bodies | cerebral neurons |
Inclusion body diseases differ from amyloid diseases in that inclusion bodies are necessarily intracellular aggregates of protein, where amyloid can be intracellular or extracellular. Amyloid also necessitates protein polymerization where inclusion bodies do not.[15]
Preventing the formation of inclusion bodies
Inclusion bodies are often made of denatured aggregates of inactive proteins. Although, the renaturation of inclusion bodies can sometimes lead to the solubilisation and the recovery of active proteins, the process is still very empirical, uncertain and of low efficiency. Several techniques have been developed over the years to prevent the formation of inclusion bodies. These techniques include:
- The use of weaker promoters to slowdown the rate of protein expression
- The use of low copy number plasmids[16]
- The co-expression of chaperone (such as GroES-GroEL and DnaK-DnaJ-GrpE)[17]
- The use of specific E. coli strains such as (AD494 and Origami)[18]
- Fusing the target protein to a soluble partner[19]
- Lowering the expression temperature
See also
- JUNQ and IPOD
- Orthopoxvirus inclusion bodies
- Inclusion body myositis
- Hereditary inclusion body myopathy
- Adult polyglucosan body disease
References
- ^ Cruts M, Gijselinck I, van der Zee J, Engelborghs S, Wils H, Pirici D, Rademakers R, Vandenberghe R, Dermaut B, Martin JJ, van Duijn C, Peeters K, Sciot R, Santens P, De Pooter T, Mattheijssens M, Van den Broeck M, Cuijt I, Vennekens K, De Deyn PP, Kumar-Singh S, Van Broeckhoven C (2006-08-24). "Null mutations in progranulin cause ubiquitin-positive frontotemporal dementia linked to chromosome 17q21". Nature. 442 (7105): 920–4. Bibcode:2006Natur.442..920C. doi:10.1038/nature05017. PMID 16862115.
- ^ Singh, Surinder Mohan; Panda, Amulya Kumar (2005-04-01). "Solubilization and refolding of bacterial inclusion body proteins". Journal of Bioscience and Bioengineering. 99 (4): 303–310. doi:10.1263/jbb.99.303. PMID 16233795.
Inclusion bodies are dense electron-refractile particles of aggregated protein found in both the cytoplasmic and periplasmic spaces of E. coli during high-level expression of heterologous protein. It is generally assumed that high level expression of non-native protein (higher than 2% of cellular protein) and highly hydrophobic protein is more prone to lead to accumulation as inclusion bodies in E. coli. In the case of proteins having disulfide bonds, formation of protein aggregates as inclusion bodies is anticipated since the reducing environment of bacterial cytosol inhibits the formation of disulfide bonds. The diameter of spherical bacterial inclusion bodies varies from 0.5–1.3 μm and the protein aggregates have either an amorphous or paracrystalline nature depending on the localization. Inclusion bodies have higher density (~1.3 mg ml−1) than many of the cellular components, and thus can be easily separated by high-speed centrifugation after cell disruption. Inclusion bodies despite being dense particles are highly hydrated and have a porous architecture.
- ^ Biochem Biophys Res Com 328(2005) 189-197
- ^ Protein Eng 7(1994) 131-136
- ^ Biochem Biophys Res Comm 312 (2003) 1383-1386
- ^ "Plant Viruses Found in Florida and Their Inclusions". University of Florida. Archived from the original on March 24, 2012.
{{cite web}}
: CS1 maint: unfit URL (link) - ^ "Inclusions of Cucumber Mosaic Cucumovirus (CMV)". University of Florida. Archived from the original on February 19, 2012.
{{cite web}}
: CS1 maint: unfit URL (link) - ^ "Inclusions of Potyviridae Found In Florida". University of Florida. Archived from the original on February 19, 2012.
{{cite web}}
: CS1 maint: unfit URL (link) - ^ "Materials and Methods for the Detection of Viral Inclusions". University of Florida. Archived from the original on February 19, 2012.
{{cite web}}
: CS1 maint: unfit URL (link) - ^ Jiang XR, Wang H, Shen Chen GQ (2015). "Engineering the bacterial shapes for enhanced inclusion bodied accumulation". Metabolic Engineering. 29: 227–237. doi:10.1016/j.ymben.2015.03.017. PMID 25868707.
- ^ Yang, Zhong, et al. "Highly efficient production of soluble proteins from insoluble inclusion bodies by a two-step-denaturing and refolding method." PloS one 6.7 (2011): e22981.
- ^ Singh, Surinder Mohan; Panda, Amulya Kumar (April 2005). "Solubilization and refolding of bacterial inclusion body proteins". Journal of Bioscience and Bioengineering. 99 (4): 303–310. doi:10.1263/jbb.99.303. ISSN 1389-1723. PMID 16233795.
- ^ Rosenzweig, Rina; Nillegoda, Nadinath B.; Mayer, Matthias P.; Bukau, Bernd (November 2019). "The Hsp70 chaperone network". Nature Reviews. Molecular Cell Biology. 20 (11): 665–680. doi:10.1038/s41580-019-0133-3. ISSN 1471-0080. PMID 31253954.
- ^ Chapter 20 in: Mitchell, Richard Sheppard; Kumar, Vinay; Abbas, Abul K.; Fausto, Nelson (2007). Robbins Basic Pathology. Philadelphia: Saunders. ISBN 978-1-4160-2973-1. 8th edition.
- ^ Ross; Poirier (2004). "Protein aggregation and neurodegenerative disease". Nature Medicine. 10 Suppl: S10-7. doi:10.1038/nm1066. PMID 15272267.
- ^ Dmowski, Michał; Jagura-Burdzy, Grazyna (2013). "Active stable maintenance functions in low copy-number plasmids of Gram-positive bacteria II. Post-segregational killing systems". Polish Journal of Microbiology. 62 (1): 17–22. doi:10.33073/pjm-2013-002. ISSN 1733-1331. PMID 23829073.
- ^ Polissi, A.; Goffin, L.; Georgopoulos, C. (August 1995). "The Escherichia coli heat shock response and bacteriophage lambda development". FEMS Microbiology Reviews. 17 (1–2): 159–169. doi:10.1111/j.1574-6976.1995.tb00198.x. ISSN 0168-6445. PMID 7669342.
- ^ Jiang, Shann-Tzong; Tzeng, Shinn-Shuenn; Wu, Wun-Tsai; Chen, Gen-Hung (2002-06-19). "Enhanced expression of chicken cystatin as a thioredoxin fusion form in Escherichia coli AD494(DE3)pLysS and its effect on the prevention of surimi gel softening". Journal of Agricultural and Food Chemistry. 50 (13): 3731–3737. doi:10.1021/jf020053v. ISSN 0021-8561. PMID 12059151.
- ^ Waugh, David S. (2016). "The remarkable solubility-enhancing power of Escherichia coli maltose-binding protein". Postepy Biochemii. 62 (3): 377–382. ISSN 0032-5422. PMID 28132493.