Antibodies with modified affinity to fcrn that promote antigen clearance

1 - 57 . (canceled) 58 . An antibody comprising an antigen-binding domain and a human FcRn-binding domain, which has a human FcRn-binding activity at pH 6.0 and at pH 7.4, and a lower antigen-binding activity at pH 6.0 than at pH 7.4, wherein the ratio of antigen-binding activity at pH 6.0 and at pH 7.4 is at least 2 in the value of KD (at pH 6.0)/KD (at pH 7.4), wherein as the human FcRn-binding domain an human Fc domain comprises M428L and N434S substitutions in EU numbering. 59 . The antibody of claim 58 , which comprises an amino acid mutation of the antigen-binding domain, which comprises a substitution of histidine for at least one amino acid of the antigen-binding domain or the insertion of at least one histidine. 60 . The antibody of claim 59 , wherein the antigen-binding domain comprises one or more substitutions selected from the following sites; Heavy chain: H27, H31, H32, H33, H35, H50, H58, H59, H61, H62, H63, H64, H65, H99, H100b, and H102 by the Kabat numbering system. 61 . The antibody of claim 60 , wherein the antigen-binding domain comprises substitution site at H27 in Heavy chain by Kabat numbering system. 62 . The antibody of claim 58 , the ratio of antigen-binding activity at pH 6.0 and at pH 7.4 is at least 40 in the value of KD (at pH 6.0)/KD (at pH 7.4). 63 . The antibody of claim 58 , which binds to a soluble antigen. 64 . The antibody of claim 63 , wherein the soluble antigen is C5. 65 . The antibody of claim 64 , wherein the antibody is selected from a chimeric antibody, a humanized antibody or a human antibody. 66 . A pharmaceutical composition comprising the antibody of claim 58 . 67 . A method for facilitating antibody-mediated antigen uptake into a cell by substituting M428L and N434S in EU numbering, in the human IgG Fc domain as the human FcRn-binding domain and reducing its antigen-binding activity at pH 6.0 to less than that at pH 7.4, wherein the antibody comprises an antigen-binding domain and a human FcRn-binding domain. 68 . A method for increasing the number of antigens to which a single antibody can bind by substituting M428L and N434S in EU numbering, in the human IgG Fc domain as the human FcRn-binding domain and reducing its antigen-binding activity at pH 6.0 to less than that at pH 7.4, wherein the antibody comprises an antigen-binding domain and a human FcRn-binding domain. 69 . A method for augmenting the ability of an antibody to eliminate an antigen from plasma by substituting M428L and N434S in EU numbering, in the human IgG Fc domain as the human FcRn-binding domain and reducing its antigen-binding activity at pH 6.0 to less than that at pH 7.4, wherein the antibody comprises an antigen-binding domain and a human FcRn-binding domain. 70 . A method for improving pharmacokinetics of an antibody by substituting M428L and N434S in EU numbering, in the human IgG Fc domain as the human FcRn-binding domain and reducing its antigen-binding activity at pH 6.0 to less than that at pH 7.4, wherein the antibody comprises an antigen-binding domain and a human FcRn-binding domain. 71 . A method for facilitating intracellular dissociation of an antigen bound to an antibody outside the cell from the antigen-binding molecule, by substituting M428L and N434S in EU numbering, in the human IgG Fc domain as the human FcRn-binding domain and reducing its antigen-binding activity at pH 6.0 to less that at pH 7.4, wherein the antibody comprises an antigen-binding domain and a human FcRn-binding domain. 72 . A method for facilitating extracellular release of the antigen-free form of an antibody taken up into a cell in an antigen-bound form, by substituting M428L and N434S in EU numbering, in the human IgG Fc domain as the human FcRn-binding domain and reducing its antigen-binding activity at pH 6.0 range to less than that at pH 7.4, wherein the antibody comprises an antigen-binding domain and a human FcRn-binding domain. 73 . A method for reducing total or free plasma antigen concentration in plasma, by substituting M428L and N434S in EU numbering, in the human IgG Fc domain as the human FcRn-binding domain and reducing its antigen-binding activity at pH 6.0 range to less than that at pH 7.4, wherein the antibody comprises an antigen-binding domain and a human FcRn-binding domain. 74 . The method of claim 67 , wherein the antigen-binding activity of the antibody at pH 6.0 is reduced to less than that at pH 7.4 by substituting histidine for at least one amino acid of the antigen-binding molecule or inserting at least one histidine. 75 . The method of claim 74 , wherein the decrease in the antigen-binding activity is represented by an increase in the value of KD (at pH 6.0)/KD (at pH 7.4) which is a ratio of antigen-binding activity at pH 6.0 and at pH 7.4, relative to before histidine substitution or insertion. 76 . A method for producing an antibody, which comprises the steps of: (a) selecting an antibody that comprises as the human FcRn-binding domain an human Fc domain comprising M428L and N434S substitutions in EU numbering; (b) altering at least one amino acid in the antigen-binding domain of an antibody and selecting an antibody that has stronger antigen-binding activity at pH7.4 than at pH 6.0; (c) obtaining a gene encoding an antibody in which a human FcRn-binding domain and an antigen-binding domain prepared in (a) and (b) are linked; and (d) producing an antibody using the gene prepared in (c). 77 . A method for producing an antibody, which comprises the steps of: (a) selecting an antibody that comprises as the human FcRn-binding domain an human Fc domain comprising M428L and N434S substitutions in EU numbering; (b) selecting an antigen-binding molecule that has stronger antigen-binding activity at pH 7.4 than at pH 6.0; (c) obtaining a gene encoding an antibody in which a human FcRn-binding domain and an antigen-binding domain prepared in (a) and (b) are linked; and (d) producing an antibody using the gene prepared in (c). 78 . An antibody produced by the production method of claim 76 .