Due to the simple
purification of this enzyme (5-30 fold purification is sufficient to reach homogeneity), its biological and biochemical analysis have been very thoroughly studied. raised
antiserum to these specific HNL, which were then applied (with
colloidal gold particles in tow) to Black Cherry
cotyledon and
endosperm. Here it was found that HNL overwhelmingly localizes to the cell walls of these developing plants. It was so enriched in these regions that it was noted upwards of 5% of the
cell wall images taken via
Electron Microscopy imaged the gold particles that were indirectly
labelling these proteins. Knowing where this protein is highly localized, Figure 1 details work that highlights the structure of this protein and the residues in its active site respectively. Of specific interest, HNLs make use of a catalytically active
Cys residue. While
Cysteine residues are conserved throughout species in three separate locations (at the
N-terminal FAD binding site, and two at the
C-terminal active site), it appears that the catalytically active residue lies near the active site, suggesting an important role in HNL catalytic action. Other structural features indicative of HNL are split based on their class. While Class II HNL are known to be more heterogenous and more often seen in
grains, Class I HNL are more typically FAD-binding and function as
seed storage proteins. This action allows for increased
amino acid metabolism in developing seeds. Because the enzyme is able to quickly reverse this reaction to create
hydrogen cyanide, HNLs play an essential role in defense of the seed As of late 2007, only one
structure has been solved for this class of enzymes, with the
PDB accession code . == Mechanism of action ==