(118a) All-Atom Molecular Dynamics Simulations of Poly-Ethylene-Glycol (PEG) and Limp-2 Reveal That Peg Penetrates Deep into the Proposed CD36 Cholesterol-Transport Tunn
AIChE Annual Meeting
2022
2022 Annual Meeting
Food, Pharmaceutical & Bioengineering Division
Biomolecular Engineering III
Monday, November 14, 2022 - 12:30pm to 12:48pm
Poly-ethylene-glycol (PEG) is the most prominent clinically administered synthetic polymer. For example, over 300M people have been administered PEGylated liposome vaccines for SARS-CoV-2. PEG is used in mammals because it has low affinity for most proteins and vice versa. However, this makes it difficult to study the few interactions with proteins that PEG has. On the atomistic level, there are two PEG-protein structures: 1) PEG-LIMP-2 and 2) PEG-aPEG. In the first structure, two monomers of a 1.5 kDA PEG polymer (PEG2) had electron density deep in the postulated cholesterol transport tunnel of LIMP-2, a lysosomal cholesterol transport protein, and member of the CD36 super family of proteins. It is unclear how PEG entered this tunnel. In the second structure, PEG wrapped around a surface-exposed tryptophan on its antibody. Since tryptophan is a rare residue, it is unclear if this PEG-Trp interaction is ubiquitous. To gain deeper mechanistic insight into PEG-protein interactions, we surrounded the LIMP-2 apo structure with 13 PEG chains of 10 monomers each (PEG10), water, and KCl and simulated the system using NAMD. One of the 13 chains penetrated LIMP-2 and came within 3 Å of PEG2. This was possible because of strong hydrogen bonding between multiple oxygens along PEG10 and Arg192, but, most importantly, the clamping of the tertiary structure on PEG10. Clamping stabilized the movements of PEG10 and the leading oxygen of PEG10 was able to penetrate LIMP-2 and head towards to position occupied by PEG2. Phe383 appears to act as a gate for objects to move through this cavity, which continues to the basal/membrane side of LIMP-2. Of all residues, PEG10 molecules had the most sustained interactions with lysine and arginine because of their strong hydrogen-bonding capabilities. These results show that the oxygens of PEG bind residues with high hydrogen bonding capabilities. However, the PEG-protein interaction is likely to be transient unless groups of resides can clamp down on PEG or a cavity that at least part of the PEG chain can enter is in close proximity to lower PEGâs entropy.