Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Pivot Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Target Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Query: EC:3.2.1.17 (
lysozyme
)
21,489
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
To elucidate hydroxyapatite-protein interaction, mutant human lysozymes in which the surface charge was modified by site-directed mutagenesis were used. Five mutant human lysozymes (K1A, K13A,
K33A
, R10A, R14A) were expressed in yeast. The chromatographic behavior of these lysozymes was studied with a HPLC hydroxyapatite column. Elution molarities of K1A and R14A mutants were greatly lowered. While Lys-13 and Arg-10 are located around Lys-1 and Arg-14, K13A and R10A mutants bound onto hydroxyapatite stronger than K1A and R14A mutants. In combination with an X-ray crystal structure of human
lysozyme
, it is concluded that the adsorbing site of human
lysozyme
is at the back of the active site and that Arg-14, Lys-1, Arg-10 and Lys-13 play important roles in binding.
...
PMID:Adsorption of human lysozyme onto hydroxyapatite. Identification of its adsorbing site using site-directed mutagenesis. 949
The positively charged lysine at the C-terminals of three long alpha-helices (5-15, 25-35, and 88-99) was replaced with alanine (K13A,
K33A
, K97A) or aspartic acid (K13D, K33D, K97D) in hen
lysozyme
by genetic engineering. The denaturation transition point (Tm) and Gibbs energy change Delta G of the mutant lysozymes decreased remarkably, suggesting that the positive charge at the C-terminals of helices is involved in the stabilization of the helix dipole. On the other hand, the non-charged asparagine at the N-terminal of the long alpha-helices (25-35 and 88-99) was replaced with negatively charged aspartic acid (N27D and N93D). The Tm and Delta G of N27D increased, suggesting that the dipole moment of the N-terminal of the helices is diminished by replacement with negatively charged amino acid strengthening the stability of the helices. The stabilities of those hen egg white lysozymes mutated at the N- or C-terminal sites of the three long alpha-helices were related with their secretion amounts in yeast (Pichia pastoris). The secretion amounts of these mutant lysozymes in yeast were closely correlated with their stability.
...
PMID:Relationship between the stability of hen egg-white lysozymes mutated at sites designed to interact with alpha-helix dipoles and their secretion amounts in yeast. 1807 Dec 53
Using random mutagenesis, we previously obtained K33N mutant
lysozyme
that showed a large lytic halo on the plate coating Micrococcus luteus. In order to examine the effects of mutation of K33N on enzyme activity, we prepared K33N and
K33A
mutant lysozymes from yeast. It was found that the activities of both the mutant lysozymes were higher than those of the wild-type
lysozyme
based on the results of the activity measurements against M. luteus (lytic activity) and glycol chitin. Moreover, 3D structures of K33N and
K33A
mutant
lysozyme
were solved by X-ray crystallographic analyses. The side chain of K33 in the wild-type
lysozyme
hydrogen bonded with N37 involved in the substrate-binding region, and the orientation of the side chain of N37 in K33 mutant lysozymes were different in the wild-type
lysozyme
. These results suggest that the enhancement of activity in K33N mutant
lysozyme
was due to an alteration in the orientation of the side chain of N37. On the other hand, K33N
lysozyme
was less stable than the wild-type
lysozyme
. Lysozyme may sacrifice its enzyme activity to acquire the conformational stability at position 33.
...
PMID:Crystal structures of K33 mutant hen lysozymes with enhanced activities. 1877 7
