Alignment of the amino acid sequences of murine, rat and human DNASE1 (SwissProt Accession numbers P49183, P21704 and P24855) and DNASE1L3 of all three species (O55070, O89107 and Q13609). Identical amino acids are boxed, and the numbering of each sequence is given on the right. Numbering at the top refers to the murine Dnase1 sequence of the mature protein (ΔSP-Dnase1). The first 21 (DNASE1) and 25 (DNASE1L3, 20 amino acids in the case of human DNASE1L3) N-terminal amino acids represent predicted signal peptides for the directed translocation into the rER. Two NLS sequences (shaded) were identified for the human DNASE1L3 protein [30]. The amino acids building the catalytic centre (
, [35]) and chelating the Mg
2+ ions in the catalytic centre (●, [35]) of the DNASE1 protein are highly conserved between DNASE1 and DNASE1L3. The same holds true for five of the seven residues identified as essential for DNA binding (*, [36]), the second disulphide bridge (S=S) and the two Ca
2+-ion-binding sites (C1/2, [37]) of DNASE1. Differences between DNASE1 and DNASE1L3 exist for the N-glycosylation sites of DNASE1 at Asn
18 and Asn
106 (
, [40]), the binding site for monomeric actin (◆, [38]) and for the first disulphide bridge (S=S) of DNASE1, which are not conserved in the DNASE1L3 proteins. In contrast with DNASE1, DNASE1L3 proteins contain an additional C-terminal domain of 21 amino acids rich in the basic amino acids lysine and arginine.