Models of protein movement
- Also called:
- Golgi complex or Golgi body
- Key People:
- Camillo Golgi
- Related Topics:
- organelle
- cisterna
- cis Golgi cisternae
- trans Golgi cisternae
- On the Web:
- CORE - Golgi Complex: Biogenesis de novo? (Oct. 29, 2024)
The way in which proteins and lipids move from the cis face to the trans face is a matter of debate, and today there exist multiple models, with quite different perceptions of the Golgi apparatus, competing to explain this movement. The vesicular transport model, for example, stems from initial studies that identified vesicles in association with the Golgi apparatus. This model is based on the idea that vesicles bud off and fuse to cisternae membranes, thus moving molecules from one cisterna to the next; budding vesicles can also be used to transport molecules back to the endoplasmic reticulum. A vital element of this model is that the cisternae themselves are stationary. In contrast, the cisternal maturation model depicts the Golgi apparatus as a far more dynamic organelle than does the vesicular transport model. The cisternal maturation model indicates that cis cisternae move forward and mature into trans cisternae, with new cis cisternae forming from the fusion of vesicles at the cis face. In this model, vesicles are formed but are used only to transport molecules back to the endoplasmic reticulum. Other examples of models to explain protein and lipid movement through the Golgi apparatus include the rapid partitioning model, in which the Golgi apparatus is viewed as being divided into separately functioning compartments (e.g., processing versus exporting regions), and the stable compartments as cisternal progenitors model, in which compartments within the Golgi apparatus are considered to be defined by Rab proteins.
History of discovery
The Golgi apparatus was observed in 1897 by Italian cytologist Camillo Golgi. In Golgi’s early studies of nervous tissue, he had established a staining technique that he referred to as reazione nera, meaning “black reaction”; today it is known as the Golgi stain. In this technique nervous tissue is fixed with potassium dichromate and then suffused with silver nitrate. While examining neurons that Golgi stained using his black reaction, he identified an “internal reticular apparatus.” This structure became known as the Golgi apparatus, though some scientists questioned whether the structure was real and attributed the find to free-floating particles of Golgi’s metal stain. In the 1950s, however, when the electron microscope came into use, the existence of the Golgi apparatus was confirmed.