Liposome

A liposome is a tiny bubble (vesicle), made out of the same material as a cell membrane. Liposomes can be filled with drugs, and used to deliver drugs for cancer and other diseases.

Membranes are usually made of phospholipids, which are molecules that have a head group and a tail group. The head is attracted to water, and the tail, which is made of a long hydrocarbon chain, is repelled by water.

In nature, phospholipids are found in stable membranes composed of two layers (a bilayer). In the presence of water, the heads are attracted to water and line up to form a surface facing the water. The tails are repelled by water, and line up to form a surface away from the water. In a cell, one layer of heads faces outside of the cell, attracted to the water in the environment. Another layer of heads faces inside the cell, attracted by the water inside the cell. The hydrocarbon tails of one layer face the hydrocarbon tails of the other layer, and the combined structure forms a bilayer.^[2]

When membrane phospholipids are disrupted, they can reassemble themselves into tiny spheres, smaller than a normal cell, either as bilayers or monolayers. The bilayer structures are liposomes. The monolayer structures are called micelles.

The lipids in the plasma membrane are chiefly phospholipids like phosphatidylethanolamine and phosphatidylcholine. Phospholipids are amphiphilic with the hydrocarbon tail of the molecule being hydrophobic; its polar head hydrophilic. As the plasma membrane faces watery solutions on both sides, its phospholipids accommodate this by forming a phospholipid bilayer with the hydrophobic tails facing each other.

Liposomes can be composed of naturally-derived phospholipids with mixed lipid chains (like egg phosphatidylethanolamine), or of pure surfactant components like DOPE (dioleoylphosphatidylethanolamine). Liposomes, usually but not by definition, contain a core of aqueous solution^[3]; lipid spheres that contain no aqueous material are called micelles, however, reverse micelles [1] can be made to encompass an aqueous environment.

Etymology

The name liposome is derived from two Greek words: 'Lipos' meaning fat and 'Soma' meaning body. A liposome can be formed at a variety of sizes as uni-lamellar or multi-lamellar construction, and its name relates to its structural building blocks, phospholipids, and not to its size. In contrast, the term Nanosome does relate to size and was coined in the early 1990s to denote special liposomes in the low nanometer range; liposome and Nanosome are not synonyms. A liposome does not necessarily have lipophobic contents, such as water, although it usually does.

Discovery

Liposomes were first described by British haematologist Dr Alec D Bangham FRS in 1961 (published 1964), at the Babraham Institute, in Cambridge. They were discovered when Bangham and R. W. Horne were testing the institute's new electron microscope by adding negative stain to dry phospholipids. The resemblance to the plasmalemma was obvious, and the microscope pictures served as the first real evidence for the cell membrane being a bilayer lipid structure.

Application

Liposomes are used for drug delivery due to their unique properties. A liposome encapsulates a region on aqueous solution inside a hydrophobic membrane; dissolved hydrophilic solutes cannot readily pass through the lipids. Hydrophobic chemicals can be dissolved into the membrane, and in this way liposome can carry both hydrophobic molecules and hydrophilic molecules. To deliver the molecules to sites of action, the lipid bilayer can fuse with other bilayers such as the cell membrane, thus delivering the liposome contents. By making liposomes in a solution of DNA or drugs (which would normally be unable to diffuse through the membrane) they can be (indiscriminately) delivered past the lipid bilayer. There are three types of liposomes - MLV (multilamillar vesicles) SUV (Small Unilamillar Vasicles) and LUV (Large Unilamillar Vesicles). These are used to deliver different types of drugs.

Liposomes are used as models for artificial cells. Liposomes can also be designed to deliver drugs in other ways. Liposomes that contain low (or high) pH can be constructed such that dissolved aqueous drugs will be charged in solution (i.e., the pH is outside the drug's pI range). As the pH naturally neutralizes within the liposome (protons can pass through some membranes), the drug will also be neutralized, allowing it to freely pass through a membrane. These liposomes work to deliver drug by diffusion rather than by direct cell fusion. Another strategy for liposome drug delivery is to target endocytosis events. Liposomes can be made in a particular size range that makes them viable targets for natural macrophage phagocytosis. These liposomes may be digested while in the macrophage's phagosome, thus releasing its drug. Liposomes can also be decorated with opsonins and ligands to activate endocytosis in other cell types.

The use of liposomes for transformation or transfection of DNA into a host cell is known as lipofection.

In addition to gene and drug delivery applications, liposomes can be used as carriers for the delivery of dyes to textiles^[4], pesticides to plants, enzymes and nutritional supplements to foods, and cosmetics to the skin ^[5].

The use of liposomes in nano cosmetology also has many benefits, including improved penetration and diffusion of active ingredients, selective transport of active ingredients, longer release time, greater stability of active, reduction of unwanted side effects, and high biocompatibility

Targeting cancer

Another interesting property of liposomes are their natural ability to target cancer. The endothelial wall of all healthy human blood vessels are encapsulated by endothelial cells that are bound together by tight junctions. These tight junctions stop any large particle in the blood from leaking out of the vessel. Tumour vessels do not contain the same level of seal between cells and are diagnostically leaky. This ability is known as the Enhanced Permeability and Retention effect. Liposomes of certain sizes, typically less than 400nm, can rapidly enter tumour sites from the blood, but are kept in the bloodstream by the endothelial wall in healthy tissue vasculature. Anti-cancer drugs such as Doxorubicin (Doxil), Camptothecin and Daunorubicin (Daunoxome) are currently being marketed in liposome delivery systems.

Manufacturing

The correct choice of liposome preparation method depends on the following parameters: 1) the physicochemical characteristics of the material to be entrapped and those of the liposomal ingredients; 2) the nature of the medium in which the lipid vesicles are dispersed; 3) the effective concentration of the entrapped substance and its potential toxicity; 4) additional processes involved during application/delivery of the vesicles; 5) optimum size, polydispersity and shelf-life of the vesicles for the intended application; and, 6) batch-to-batch reproducibility and possibility of large-scale production of safe and efficient liposomal products ^[6] ^[7]. It should be noted that formation of liposomes and nanoliposomes is not a spontaneous process. Lipid vesicles are formed when phospholipids such as lecithin are placed in water and consequently form one bilayer or a series of bilayers, each separated by water molecules, once enough energy is supplied ^[8]. Liposomes can be created by sonicating phospholipids in water^[3]. Low shear rates create multilamellar liposomes, which have many layers like an onion. Continued high-shear sonication tends to form smaller unilamellar liposomes. In this technique, the liposome contents are the same as the contents of the aqueous phase. Sonication is generally considered a "gross" method of preparation as it can damage the structure of the drug to be encapsulated. Newer methods such as extrusion and Mozafari method ^[9] are employed to produce materials for human use.

Prospect

Further advances in liposome research have been able to allow liposomes to avoid detection by the body's immune system, specifically, the cells of reticuloendothelial system (RES). These liposomes are known as "stealth liposomes", and are constructed with PEG (Polyethylene Glycol) studding the outside of the membrane. The PEG coating, which is inert in the body, allows for longer circulatory life for the drug delivery mechanism. However, research currently seeks to investigate at what amount of PEG coating the PEG actually hinders binding of the liposome to the delivery site. In addition to a PEG coating, most stealth liposomes also have some sort of biological species attached as a ligand to the liposome in order to enable binding via a specific expression on the targeted drug delivery site. These targeting ligands could be monoclonal antibodies (making an immunoliposome), vitamins, or specific antigens. Targeted liposomes can target nearly any cell type in the body and deliver drugs that would naturally be systemically delivered. Naturally toxic drugs can be much less toxic if delivered only to diseased tissues. Polymersomes, morphologically related to liposomes can also be used this way.

References

^ Torchilin VP. (2006)Adv Drug Deliv Rev. 2006 Dec 1;58(14):1532-55
^ Kimball's Biology Pages, "Cell Membranes."
^ ^a ^b Stryer S. (1981) Biochemistry, 213
^ Barani, H. & Montazer, M. (2008) A Review on Applications of Liposomes in Textile Processing. Journal of Liposome Research, 18 (3) 249-262
^ Meure, L.A., Knott, R., Foster, N.R., Dehghani, F. (2009) The Depressurization of an Expanded Solution into Aqueous Media for the Bulk Production of Liposomes. Langmuir, 25, 326-337
^ Gomez-Hens, A., Fernandez-Romero, J.M. (2006). Analytical methods for the control of liposomal delivery systems. Trends Anal Chem 25:167–178.
^ Mozafari, M.R., Johnson, C., Hatziantoniou, S. & Demetzos, C. (2008) Nanoliposomes and their applications in food nanotechnology. Journal of Liposome Research. 18 (4), 309-327.
^ Mozafari, M.R. & Mortazavi, S.M. (2005) Nanoliposomes: From Fundamentals to Recent Developments. Trafford Publishing Ltd, Oxford, UK.
^ Colas, J.C., Shi, W.L., Rao, V.S.N.M., Omri, A., Mozafari, M.R., Singh, H. (2007) Microscopical investigations of nisin-loaded nanoliposomes prepared by Mozafari method and their bacterial targeting. Micron 38:841–847.

External links

[1] Torchilin VP. (2006)Adv Drug Deliv Rev. 2006 Dec 1;58(14):1532-55

[2] Kimball's Biology Pages, "Cell Membranes."

[Stryer_S._1981_Biochemistry,_213-3] Stryer S. (1981) Biochemistry, 213

[4] Barani, H. & Montazer, M. (2008) A Review on Applications of Liposomes in Textile Processing. Journal of Liposome Research, 18 (3) 249-262

[5] Meure, L.A., Knott, R., Foster, N.R., Dehghani, F. (2009) The Depressurization of an Expanded Solution into Aqueous Media for the Bulk Production of Liposomes. Langmuir, 25, 326-337

[6] Gomez-Hens, A., Fernandez-Romero, J.M. (2006). Analytical methods for the control of liposomal delivery systems. Trends Anal Chem 25:167–178.

[7] Mozafari, M.R., Johnson, C., Hatziantoniou, S. & Demetzos, C. (2008) Nanoliposomes and their applications in food nanotechnology. Journal of Liposome Research. 18 (4), 309-327.

[8] Mozafari, M.R. & Mortazavi, S.M. (2005) Nanoliposomes: From Fundamentals to Recent Developments. Trafford Publishing Ltd, Oxford, UK.

[9] Colas, J.C., Shi, W.L., Rao, V.S.N.M., Omri, A., Mozafari, M.R., Singh, H. (2007) Microscopical investigations of nisin-loaded nanoliposomes prepared by Mozafari method and their bacterial targeting. Micron 38:841–847.

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