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Review
. 2010 Sep;2(9):a002212.
doi: 10.1101/cshperspect.a002212. Epub 2010 May 19.

The origins of cellular life

Affiliations
Review

The origins of cellular life

Jason P Schrum et al. Cold Spring Harb Perspect Biol. 2010 Sep.

Abstract

Understanding the origin of cellular life on Earth requires the discovery of plausible pathways for the transition from complex prebiotic chemistry to simple biology, defined as the emergence of chemical assemblies capable of Darwinian evolution. We have proposed that a simple primitive cell, or protocell, would consist of two key components: a protocell membrane that defines a spatially localized compartment, and an informational polymer that allows for the replication and inheritance of functional information. Recent studies of vesicles composed of fatty-acid membranes have shed considerable light on pathways for protocell growth and division, as well as means by which protocells could take up nutrients from their environment. Additional work with genetic polymers has provided insight into the potential for chemical genome replication and compatibility with membrane encapsulation. The integration of a dynamic fatty-acid compartment with robust, generalized genetic polymer replication would yield a laboratory model of a protocell with the potential for classical Darwinian biological evolution, and may help to evaluate potential pathways for the emergence of life on the early Earth. Here we discuss efforts to devise such an integrated protocell model.

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Figures

Figure 1.
Figure 1.
A simple protocell model based on a replicating vesicle for compartmentalization, and a replicating genome to encode heritable information. A complex environment provides lipids, nucleotides capable of equilibrating across the membrane bilayer, and sources of energy (left), which leads to subsequent replication of the genetic material and growth of the protocell (middle), and finally protocellular division through physical and chemical processes (right). (Reproduced from Mansy et al. 2008 and reprinted with permission from Nature Publishing ©2008.)
Figure 2.
Figure 2.
Vesicle shape transformations during growth. All vesicles are labeled with 2 mM encapsulated HPTS, a water-soluble fluorescent dye, in their internal aqueous space. (A) 10 min and (B) 30 min after the addition of five equivalents of oleate micelles to oleate vesicles (in 0.2 M Na-bicine, pH 8.5). Scale bar: 50 µm. (Reproduced from Zhu and Szostak 2009a and reprinted with permission from ACS Publications ©2009.)
Figure 3.
Figure 3.
Schematic diagram of coupled vesicle growth and division. (Reproduced from Zhu and Szostak 2009a and reprinted with permission from the Journal of the American Chemical Society ©2009.)
Figure 4.
Figure 4.
Structures of 2′-5′ phosphoramidate DNA, and the corresponding activated monomers.
Figure 5.
Figure 5.
Watson Crick base-pairs. Top: Standard A:U base-pair. Bottom: Alternative diaminopurine (D): C5-propynyl-uracil (Up) base-pair.

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