Inactivation ofhuman eystatin C and kininogen by human cat, hepsin D Univcrslt, v th~sptml, S.221 85 l.und, 3"wcdcn Received i 6 Janultry 1991 A p~p~ln tnltibitor of 22 kDa was isolated from human pt=te=nta and shown to ~ identical to residues Cy~146.keu:t?.~ of the third domain of human klninol~en. This kinino~en dam;tin anti reeon~binan~ hun~an cystatin C were tmtettvated by pcptlde bond eleavalles at hydrophobic amino acid residues due to Ihe etClion of cathepsin D, Tlie~e results ftmher support 11~c prop=seal role ofcalhepsin D in the regulation orcysteinc proteinus~ activity. In this report we show that cathepsin D is able to degrade human cystatin C and the third domain of kininogen, both extracell.ular protein inhibitors of cysteine proteinases. This finding might be important for elucidation of additional e×tracellular actions of cathepsin D.
MATERIALS AND METHODS
2,1 MaterialsRecombinant human cystatin C was prepared as described [13]. Human cathepsin D was isolated from spleen [14], Papain (type 111) (EC 3,4,22,2) and sttbstrate BANA were from Sigma, Bovine haemoglobin was prepared as described in [15]. Pepstatin was from Peptide Research Foundation (Osaka, Japan). Acetonitrile and t rifluoroacetic acid were from Merck and BDH Chemicals, respectively. All other chemicals were of analytical grade,
Isnlatlan of thv third don~ain af kinhlogc, nThe isolation was carried out followinj tile procedure as described in [161 with some modirietttions. Briefly, human placenta (1000 g) was homogenized in 0.9~, NaCI (I :1.5, w/v) sohnlon and centrifuged for 60 rain a= 14 000 x /~. The supernatant war adjusted to pet 10,$ with 5 M NaOH, and after standing I h at roan1 temperature, to pH ?.S with 3 M HCI, After ¢entrifugation the supernatant was applied to an affinity column (7.5 × $.0 era) of Cm-papain-Sepharose 4B prepared as in [1"7], et|uilibrated with 10 mM Tris-HCI buffer (pH 7.5). The coluntn was washed with the same t~uffer and the bomtd proteins eluted tl~en with 10 mM NaOH (pH I 1.01, Papain.inhibitlng fractions were pooled, adjusted to pH g.O with 3 M HCI and concentrated by ultrafiltration on an YM-5 membrane (Amicon). The concentrated sample war dialyzed against 10 mM Tris-HCI buffer (pH 7,5) containing 0,1 M NaCI and applied to a column (120 x 5 cm) of Sephadex G-75 equilibrated in the same buffer, Papain.inhihiting fractions were resolved as three peaks corresponding to M, of about 12 25 attd 6S kDa, The 25 kDa.M, protein peak was dialyzed against 10 mM Tris-HCI buffer (pH 8,5) at~d subsequently cllromatographed on DEAESephacel eq uilibrated with the same buffer, The inhibitor was eluted in a single symmetrical peak with linear gradient of NaCI (0,05-0,15 M) in the same buffer, The sample was concentrated, assayed for its purity by SDS-PAGE and amino acid sequence analysis, and stored at -25"C until use,
2,3. Assays of enzymes and inhibitorsThe inhibitory activity of cystatin C and the third domain of kininogen was determined by measuring the inhibition of papain using BANA as substrate [18], The c...
