12098354 (P.T.A.B. Jan. 18, 2018)

Ex Parte Alexis et al

Patent Trial and Appeal BoardJan 18, 2018

12098354 (P.T.A.B. Jan. 18, 2018)

United States Patent and Trademark Office UNITED STATES DEPARTMENT OF COMMERCE United States Patent and Trademark Office Address: COMMISSIONER FOR PATENTS P.O.Box 1450 Alexandria, Virginia 22313-1450 www.uspto.gov APPLICATION NO. FILING DATE FIRST NAMED INVENTOR ATTORNEY DOCKET NO. CONFIRMATION NO. 12/098,354 04/04/2008 Frank Alexis MIT 12388 2137 23579 7590 Pabst Patent Group LLP 1545 PEACHTREE STREET NE SUITE 320 ATLANTA, GA 30309 EXAMINER CRAIGO, WILLIAM A ART UNIT PAPER NUMBER 1615 MAIL DATE DELIVERY MODE 01/18/2018 PAPER Please find below and/or attached an Office communication concerning this application or proceeding. The time period for reply, if any, is set in the attached communication. PTOL-90A (Rev. 04/07) UNITED STATES PATENT AND TRADEMARK OFFICE BEFORE THE PATENT TRIAL AND APPEAL BOARD Ex parte FRANK ALEXIS, LIANGFANG ZHANG, ALEKSANDAR F. RADOVIC-MORENO, FRANK X. GU, PAMELA BASTO, ETGAR LEVY-NISSENBAUM, JULIANA CHAN, ROBERT S. LANGER, and OMID C. FAROKHZAD1 Appeal 2016-008166 Application 12/098,354 Technology Center 1600 Before DONALD E. ADAMS, ERIC B. GRIMES, and JOHN E. SCHNEIDER, Administrative Patent Judges. GRIMES, Administrative Patent Judge. DECISION ON APPEAL This is an appeal under 35 U.S.C. § 134 involving claims to a dosage unit formulation, which have been rejected as lacking adequate written description and as obvious. We have jurisdiction under 35 U.S.C. § 6(b). We affirm. 1 Appellants identify the Real Parties in Interest as Massachusetts Institute of Technology; The Brigham and Women’s Hospital, Inc.; Bind Biosciences, Inc.; and Selecta Biosciences, Inc. (Appeal Br. 2.) Appeal 2016-008166 Application 12/098,354 STATEMENT OF THE CASE “Nanoparticles have been developed as vehicles used in the administration for the delivery of small molecule drugs as well as proteins, peptide drugs and nucleic acids. The drugs are typically encapsulated or conjugated in a polymer matrix. ... As the polymer is degraded and/or as the drug diffuses out of the polymer, the drug is released into the body.” (Spec. 1:30 to 2:1.) “Targeting controlled release polymer systems (e.g., targeted to a particular tissue or cell type or targeted to a specific diseased tissue but not normal tissue) is desirable because it reduces the amount of a drug present in tissues of the body that are not targeted.” (Id. at 2:7—10.) The Specification discloses nanoparticles having poly(amino acid) targeting moieties that are effective in treating vulnerable plaque, cancer, or restenosis. (Id. at 3:10-18.) The poly(amino acid) can be, for example, a glycoprotein, protein, peptidomimetic, affibody, or peptide. (Id. at 3:25—29.) “The term ‘affibody’ . . . refers to highly specific affinity proteins that can be designed to bind to any desired target molecule.” (Id. at 29:15—17.) Claims 1, 2, 4, 7, 8, 13, 15, 16, 20-22, 24, 25, 28, 46-A8, 63, and 82- 84 are on appeal. Claim 1 is illustrative and reads as follows: 1. A dosage unit formulation comprising polymeric target-specific nanoparticles for use in treating vulnerable plaque, cancer, or restenosis, comprising an effective amount of a therapeutic, prophylactic or diagnostic agent for the treatment of vulnerable plaque, cancer, or restenosis, wherein the nanoparticles have attached thereto poly(amino acid) targeting moieties that selectively bind (i) collagen in the basement membrane of a blood vessel attached thereto, (ii) injured vasculature, or (iii) HER2. 2 Appeal 2016-008166 Application 12/098,354 The claims stand rejected as follows: Claims 1, 2, 4, 7, 8, 15, 16, 20-22, 24, 25, 28, 46-48, 63, and 82-84 under 35U.S.C. § 112, first paragraph, for lack of adequate written description (Final Action2 10); Claims 1, 2, 4, 7, 8, 15, 16, 20-22, 24, 25, 48, 63, and 82—84 under 35 U.S.C. § 103(a) as obvious based on Farokhzad,3 Lanza,4 and Ruoslahti5 (Final Action 22); Claims 46-48 under 35 U.S.C. § 103(a) as obvious based on Farokhzad, Lanza, Ruoslahti, and Hoarau6 (Final Action 27); Claims 25, 28, and 83 under 35 U.S.C. § 103(a) as obvious based on Farokhzad, Lanza, Ruoslahti, and Duncanson7 (Final Action 28); and Claim 13 under 35 U.S.C. § 103(a) as obvious based on Farokhzad, Lanza, Ruoslahti, and Chhatwal8 (Final Action 30). I The Examiner has rejected claims 1, 2, 4, 7, 8, 15, 16, 20—22, 24, 25, 28, 46-48, 63, and 82—84 for lack of adequate written description, on the basis that “[t]he number of polyamino acid targeting species disclosed does 2 Office Action mailed May 15, 2015. 3 Farokhzad et al., US 2005/0037075 Al, published Feb. 17, 2005. 4 Lanza et al., US 2004/0115192 Al, published June 17, 2004. 5 Ruoslahti et al., US 2005/0048063 Al, published Mar. 3, 2005. 6 Hoarau et al., US 2005/0214378 Al, published Sept. 29, 2005. 7 Duncanson et al., Targeted binding ofPLA microparticles with lipid-PEG- tethered ligands, 28 Biomaterials 4991 4999 (2007). 8 Chhatwal et al., WO 2007/140953 Al, published Dec. 13, 2007. 3 Appeal 2016-008166 Application 12/098,354 not constitute support for a claim to the entire genus of polyamino acid targeting moieties that are claimed functionally.” (Final Action 11.) The Examiner finds that “[t]he claims are genus claims, encompassing any poly(amino acid) of any sequence and length, which functions to provide desired properties,” and therefore are “extremely broad, in that other than being a polyamino acid, no structure is required of the targeting moieties.” (Id. at 12—13.) The Examiner finds that the Specification describes two peptides, with the sequences ARYLQKLN and AKERC, that bind respectively to injured vasculature and extracellular basement membranes, and states that anti-Her2-affibody binds to HER2, although no structural description is provided for the anti-Her2-affibody. (Id. at 14.) The Examiner finds that the Specification states that the peptide CREKA also binds to injured vasculature. (Id. at 16.) The Examiner also finds that, “[ojther than the particular polyamino acid sequences . . . AKERC, CREKA, ARYLQKLN or AXYLZZLN, wherein X and Z are variable amino acids, there do not appear to be any other particular species of poly(amino acids) disclosed by specific structures which are effective to achieve the claimed functions.” (Id.) The Examiner concludes that “[t]he specification does not demonstrate that the applicant has made a generic invention that achieves the claimed result by showing that the applicant has invented species sufficient to support a claim to the functionally-defined genus of polyamino acid targeting moieties,” and does not show that Appellants were in possession of the claimed invention at the time the application was filed. (Id. at 18.) 4 Appeal 2016-008166 Application 12/098,354 We agree with the Examiner that a person of ordinary skill in the art would not have recognized that Appellants were in possession of the claimed genera based on the written description provided in the Specification. “[T]he test for sufficiency [of written description] is whether the disclosure of the application relied upon reasonably conveys to those skilled in the art that the inventor had possession of the claimed subject matter as of the filing date.” AriadPharms., Inc. v. EliLilly & Co., 598 F.3d 1336, 1351 (Fed. Cir. 2010). A “sufficient description of a genus instead requires the disclosure of either a representative number of species falling within the scope of the genus or structural features common to the members of the genus so that one of skill in the art can ‘visualize or recognize’ the members of the genus.” Id. at 1350. “One needs to show that one has truly invented the genus, i.e., that one has conceived and described sufficient representative species encompassing the breadth of the genus. Otherwise, one has only a research plan, leaving it to others to explore the unknown contours of the claimed genus.” AbbVie Deutschland GmbH & Co. v. Janssen Biotech, Inc., 759 F.3d 1285, 1300 (Fed. Cir. 2014). Here, claim 1 reads on a formulation comprising nanoparticles with attached poly(amino acid) targeting moieties that selectively bind to (i) collagen in the basement membrane of an attached blood vessel, (ii) injured vasculature, or (iii) HER2. The Specification states that a “poly(amino acid)” can comprise natural amino acids, unnatural amino acids, modified amino acids, protected amino acids, or a mimetic of amino acids. (Spec. 3:25—27.) The Specification also states that a “poly(amino 5 Appeal 2016-008166 Application 12/098,354 acid)” can be a glycoprotein, a protein, a peptidomimetic, an affibody, or a peptide. (Id. at 3:27—29.) The scope of the poly(amino acid) targeting moieties encompassed by claim 1 is therefore very broad. The encompassed targeting moieties can comprise any of the types of amino acids, and can be any of the types of amino acid-based compounds, that are recited in the Specification. The Specification describes five specific targeting moieties: anti- HER2 affibody, AKERC, CREKA, ARYLQKLN or AXYLZZLN, wherein X and Z are variable amino acids. (Id. at 4:1 4.) The Specification states that CREKA and AXYLZZLN (which includes the peptide ARYLQKLN) bind to extracellular basement membranes under atherosclerotic plaques. (Id. at 78:31 to 79:9.) The Specification states that AKERC binds to collagen IV in extracellular basement membranes. (Id. at 82:22—23.) The Specification does not describe other poly(amino acid) targeting moieties that bind to HER2 or that bind to extracellular basement membranes, either attached to a blood vessel or in injured vasculature. We agree with the Examiner that the limited number of species that are structurally described in the Specification for the poly(amino acid) targeting moieties recited in claim 1 are not representative of the full scope of the recited genera of those moieties. The Specification does not describe structural features of poly(amino acid) targeting moieties that are common to those binding to HER2 or those binding to extracellular basement membranes. Thus, the Specification does not provide a written description of the recited genera in terms “so that one of skill in the art can ‘visualize or recognize’ the members of the genus.” 6 Appeal 2016-008166 Application 12/098,354 Ariad, 598 F.3d at 1350. The Specification therefore does not adequately describe the genera of poly(amino acid) targeting moieties that are recited in claim 1 adequately to show that Appellants were in possession of the full scope of the claimed formulation at the time the instant application was filed. Appellants argue that the Specification describes the recited poly(amino acid) targeting moieties at page 29, lines 28—30; Examples 4 and 8; and Figures 19 and 20. (Appeal Br. 12—13.) We have reviewed the cited portions of the Specification and Figures, but are not persuaded that they adequately describe the recited genera. The Specification at page 29, lines 28—30 states that “the invention provides a nanoparticle conjugated to a poly(amino acid) that selectively targets tumor vasculature and that selectively binds the alpha 2 chain of collagen IV.” The Specification’s Example 4 describes the peptide AKERC. (Spec. 81:31 to 83:2.) The Specification’s Example 8 describes “anti-HER-2 [ajffibody.” (Id. at 89:32.) Figures 19 and 20 both describe the peptide ARYLQKLN. The cited disclosures therefore describe nothing beyond the particular species that are discussed above, and that are inadequate to show possession of the full scope of the recited genera. In the Reply Brief, Appellants argue that the Examiner erred in finding that the level of predictability for the claimed targeting moieties is very low, because “the skilled person would understand the CEAKR peptide was deliberately used by Appellants as a negative control to demonstrate the 7 Appeal 2016-008166 Application 12/098,354 efficacy of the CREKA peptide to selectively localize the claimed nanoparticles to collagen IV.” (Reply Br. 7.9) This argument does not persuade us that the rejection should be reversed. Regardless of whether the peptide CEAKR would be expected to direct nanoparticles to collagen IV, claim 1 encompasses, among other things, any poly(amino acid) targeting moiety that binds to any target in the collagen of the basement membrane attached to a blood vessel or any target in injured vasculature. We agree with the Examiner that the Specification’s examples are inadequate to allow those of ordinary skill in the art to predict with reasonable assurance which poly(amino acid) targeting moieties other than those species described in the Specification would bind to the recited targets. We therefore affirm the rejection of claim 1 under 35 U.S.C. § 112, first paragraph. Claims 2, 4, 7, 8, 15, 16, 20-22, 24, 25, 28, 46-48, 63, and 82—84 have not been argued separately and fall with claim 1. 37 C.F.R. § 41.37(c)(l)(iv). 9 The Reply Brief also presents new arguments based on the state of the art at the time of filing and the description of the molecular targets bound by the recited targeting moieties. (Reply Br. 3—7 and 8—11.) These arguments were not presented in the Appeal Brief and are not responsive to anything in the Examiner’s Answer. Therefore, we will not consider them. See 37 C.F.R. § 41.41(b)(2) (“Any argument raised in the reply brief which was not raised in the appeal brief, or is not responsive to an argument raised in the examiner’s answer, including any designated new ground of rejection, will not be considered by the Board for purposes of the present appeal.”). 8 Appeal 2016-008166 Application 12/098,354 II The Examiner has rejected claims 1, 2, 4, 7, 8, 15, 16, 20—22, 24, 25, 48, 63, and 82—84 as obvious based on Farokhzad, Lanza, and Ruoslahti. The Examiner finds that “Farokhzad teaches a pharmaceutically acceptable formulation comprising polymeric target specific nanoparticles comprising a therapeutic, prophylactic or diagnostic agent.” (Final Action 22.) The Examiner finds that Farokhzad does not teach a poly(amino acid) targeting moiety, but Lanza teaches that antibodies, peptides, and nucleic acids were all “known in the art as targeting moieties and equivalent for the purpose of improving delivery of therapeutic agent.” (Id. at 24.) The Examiner concludes that it would have been obvious to modify Farokhzad’s formulation to include a poly(amino acid) targeting moiety because doing so would simply require substitution of one known targeting moiety for another. (Id.) The Examiner finds that Ruoslahti teaches poly(amino acid) targeting moieties that selectively bind collagen in the vascular basement membrane. (Id. at 25.) The Examiner finds that Ruoslahti also teaches that its targeting moieties home therapeutic agents to vasculature, are useful for improving cancer treatment, and reduce side effects. (Id.) The Examiner concludes that these teachings would have led a skilled artisan to modify Farokhzad’s formulation to include the specific poly(amino acid) targeting moieties disclosed by Ruoslahti. We agree with the Examiner that the formulation of claim 1 would have been obvious based on the cited references. Farokhzad discloses “a conjugate that includes a nucleic acid ligand bound to a controlled release 9 Appeal 2016-008166 Application 12/098,354 polymer system [and] a pharmaceutical composition that contains the conjugate.” (Farokhzad 1 8.) Farokhzad states that “[t]he controlled release polymer system includes an agent such as a therapeutic, diagnostic, prognostic, or prophylactic agent. The nucleic acid ligand that is bound to the controlled release polymer system, binds selectively to a target, such as a cell surface antigen.” (Id.) Farokhzad states that “[t]he nucleic acid ligands are DNA or RNA oligonucleotides. . . . Like antibodies, nucleic acid ligands can be prepared that bind to target antigens with high specificity and affinity and thus can be used as targeting vehicles.” (Id. 112.) Lanza discloses a composition for delivering a bioactive agent to targeted tissues or cells that comprises a site-specific targeting ligand. (Lanza ^fl[ 22—23.) Lanza states that the targeting ligand “bind[s] to molecular epitopes, ie, receptors, lipids, peptides, cell adhesion molecules, polysaccharides, biopolymers, and the like.” (Id. 131.) Lanza also states that a “wide variety of ligands, including but not limited to antibodies, antibody fragments, peptides, small molecules, polysaccharides, nucleic acids, aptamers, peptidomimetics, other mimetics and drugs alone or in combination may be utilized to specifically bind to cellular epitopes and receptors.” (Id.) Ruoslahti discloses “a conjugate that contains a therapeutic agent linked to a homing peptide or peptidomimetic containing the amino acid sequence CREKA (SEQ ID NO: 1), or a conservative variant or peptidomimetic thereof, that selectively homes to tumor vasculature and selectively binds collagen.” (Ruoslahti 111.) More specifically, Ruoslahti discloses that “a collagen IV alpha-2 chain related polypeptide can act as a 10 Appeal 2016-008166 Application 12/098,354 receptor for the CREKA (SEQ ID NO: 1) tumor homing peptide.” (Id. 151.) Ruoslahti states that collagen IV is “also known as ‘basement membrane collagen’ . . . and is found in the basement membrane of virtually all blood vessels.” (Id. 1 54.) These disclosures would have made obvious the formulation of claim 1. Farokhzad discloses a formulation like that of claim 1, except that its nanoparticles include a nucleic acid targeting ligand and Farokhzad does not disclose a targeting ligand that selectively binds to one of the targets recited in claim 1. However, Lanza discloses that targeting ligands that bind molecular epitopes include, among other things, peptides and nucleic acids. A person of ordinary skill in the art therefore would have understood that a peptide-based targeting ligand is functionally equivalent to a nucleic acid- based targeting ligand, and would have reasonably expected that Farokhzad’s formulation would also selectively bind to its target using a peptide targeting ligand. Ruoslahti discloses that the peptide CREKA binds to collagen IV in the basement membrane of blood vessels, and can direct a therapeutic agent to tumor vasculature. A skilled artisan therefore would have had reason to substitute Ruoslahti’s CREKA targeting peptide for the nucleic acid targeting moiety disclosed by Farokhzad with a reasonable expectation that CREKA would direct a therapeutic agent to tumor vasculature and be useful in treating cancer. Appellants argue that “[njothing in Farokhzad leads one to substitute polyamino acid ligands for aptamers. Indeed, one is led to believe that aptamers have greater specificity and affinity than proteins such as 11 Appeal 2016-008166 Application 12/098,354 antibodies, and are therefore preferred. . . . Accordingly, Farokhzad does not lead one skilled in the art to look for alternative targeting ligands.” (Appeal Br. 23—24.) Similarly, Appellants argue that “Farokhzad discourages the use of polypeptides, such as antibodies and antibody fragments as targeting moieties” and “Lanza does not describe any advantages of using poly(amino acids) over nucleic acids.” (Id. at 28.) These arguments are unpersuasive, because the rejection is based on the combined teachings of Farokhzad, Lanza, and Ruoslahti. As discussed above, Lanza teaches that peptide-based targeting moieties are functionally equivalent to the nucleic acid-based targeting moieties specifically taught by Farokhzad. While Farokhzad teaches that its nucleic acid-based targeting moieties have some advantages compared to antibodies, the Examiner’s rejection is based on substituting Ruoslahti’s CREKA peptide, not an antibody, for Farokhzad’s nucleic acids. Appellants also argue that “Ruoslahti describes a five amino acid sequence (specifically, CREKA), which interacts with all forms of collagen, including helical collagen, non-helical collagen and denatured collagen.” (Appeal Br. 25.) Appellants specifically argue that, “[bjased on the definition of ‘collagen’ set forth in paragraph [0009] [sic, 1 56] of Ruoslahti, the skilled person would understand the disclosure of Ruoslahti does not describe a ligand that selectively binds collagen in the basement membrane of a blood vessel, as claimed.” (Id. at 26.) This argument is also unpersuasive. Ruoslahti expressly states that “a collagen IV alpha-2 chain related polypeptide can act as a receptor for the CREKA (SEQ ID NO: 1) tumor homing peptide.” (Ruoslahti 151.) 12 Appeal 2016-008166 Application 12/098,354 Ruoslahti provides a working example demonstrating that “the observed interaction between CREKA (SEQ ID NO: 1) and the collagen IV fragment SEQ ID NO: 2 was specific” and concludes that its results “demonstrate that the CREKA (SEQ ID NO: 1) peptide binds a collagen IV a-2 chain related protein and further indicate that collagen IV or a related collagen can act as a receptor for tumor homing molecules in tumor vasculature.” {Id. 135, 142.) Appellants’ reliance on Ruoslahti’s paragraph 56 does not persuade us that the CREKA peptide is not specific for collagen IV in the basement membrane of blood vessels, because paragraph 56 does not expressly address the binding specificity of CREKA. Rather, paragraph 56 refers to “[t]he tumor homing molecules useful in the invention.” {Id. ]f 56.) As discussed above, however, Ruoslahti expressly discloses that CREKA is specific for collagen IV, also known as “basement membrane collagen.” {See id. H 51, 54.) Appellants argue that “formulating polymer/nucleic acid conjugates requires specific classes of polymers {e.g., non-cationic polymers) in order to facilitate the interactions required for this system.” (Appeal Br. 29.) Appellants cite Farokhzad’s disclosure that polymers with a positive surface charge may decrease specific binding of a nucleic acid ligand to its target. {Id.) Appellants conclude that “the skilled artisan would recognize from Farokhzad that polymers that are selected to meet the requirements of the system including the nucleic acids of Farokhzad would not be same as those selected to employ the poly(amino acid) targeting elements as claimed.” {Id.) 13 Appeal 2016-008166 Application 12/098,354 This argument is also unpersuasive. The Examiner’s rejection is based on replacing the nucleic acid targeting moiety disclosed by Farokhzad with the CREKA peptide targeting moiety disclosed by Ruoslahti. Thus, a skilled artisan would have recognized that Farokhzad’s disclosure of polymers that can be used with nucleic acid targeting moieties would not apply to nanoparticles having peptide-based targeting moieties. In any event, Appellants have provided no persuasive basis for concluding that the polymers that Farokhzad discloses as useful with nucleic acid targeting moieties would not also be useful with a peptide targeting moiety such as CREKA. Appellants also argue that “there is unpredictability in the results one of ordinary skill in the art would expect in formulating polymer conjugates for targeting specific tissues” and “the skilled artisan would not have a reasonable expectation of success in substituting one class of binding moieties with a different class of moieties.” (Appeal Br. 30.) This argument is also unpersuasive, because Ruoslahti expressly discloses that its CREKA peptide “selectively binds collagen,” that CREKA is a “tumor homing peptide,” and that CREKA “binds a collagen IV a-2 chain related protein.” (Ruoslahti || 11, 51, 142.) Thus, regardless of whether a skilled artisan would have been able to predict the binding specificity of other peptides, the cited evidence provides a reasonable basis for expecting that CREKA would bind to collagen IV in the basement membrane of blood vessels. 14 Appeal 2016-008166 Application 12/098,354 Finally, Appellants argue that “Simberg[10] . . . describes aNP [nanoparticle] containing the same peptide sequence CREKA. However, Simberg shows that the NP-CREKA conjugate targets clotted blood plasma proteins in tumor stroma and vasculature.” (Appeal Br. 30.) Appellants conclude that, “[t]aken together, Ruoslahti and Simberg describe an instance wherein, the conjugation of a ligand known to perform a specific function (targeting collagen IV) to a NP can result in a different property (targeting clotted blood plasma proteins).” (Id.) This argument is also unpersuasive. Simberg does not support Appellants’ position that attaching a ligand to a nanoparticle can result in different binding properties. Simberg discloses that “the CREKA peptide with a fluorescent dye attached . . . bound to clotted plasma proteins in vitro.'1'’ (Simberg 932, right col.) Simberg describes “coupling] fluorescein- labeled CREKA . . . onto the surface of 50-nm superparamagnetic, amino dextran-coated iron oxide (SPIO) nanoparticles.” (Id. at 933, left col.) Simberg states that “[t]he CREKA-SPIO nanoparticles bound to mouse and human plasma clots in vitro. . . . These results show that the particle-bound peptide retains its binding activity toward clotted plasma proteins.” (Id. at 933, left col.) Thus, Simberg discloses that the binding specificity of the CREKA peptide is the same regardless of whether it is coupled to a nanoparticle. Simberg does not support Appellants’ position that conjugating a ligand to a nanoparticle can result in a different targeting property. 10 Simberg et al., Biomimetic amplification of nanoparticle homing to tumors, 104 PNAS 932-936 (2007). 15 Appeal 2016-008166 Application 12/098,354 Appellants argue that: The examiner has identified no art disclosing the additional features of the targeting moieties of claims 7, 8, and 82. The examiner has cited no art disclosing blends of functionalized and non-functionalized polymers with altered rates of clearance nor having a lipid monolayer or amphiphilic shell, as defined by claims 83 and 84. The examiner has cited no art disclosing the agents defined by any of claims 46, 47 or 48. Nothing therefore would lead one skilled in the art to any of these claimed formulations. (Appeal Br. 27.) We disagree. Ruoslahti discloses the targeting moiety CREKA, which is a peptide (claim 8), comprising natural amino acids (claim 7), and designed to bind to a target molecule (claim 82). Claims 46 and 47 are not included in this rejection. Regarding claim 48, Ruoslahti discloses that paclitaxel is suitable for use in its method. (Ruoslahti | 80.) Regarding claim 83, the Examiner cited Farokhzad’s disclosure at || 98—101, which discusses PEGylated poly(lactic acid) nanoparticles. (See Final Action 23.) Appellants’ Specification states that a “polymer (e.g., copolymer, e.g., block copolymer) containing polyethylene glycol) repeat units is also referred to as a ‘PEGylated’ polymer. Such polymers . . . lower the rate of clearance from the circulatory system via the reticuloendothelial system (RES), due to the presence of the polyethylene glycol) groups.” (Spec. 17:15—20.) Regarding claim 84, the Examiner finds that “Farokhzad teaches the nanoparticles comprising an amphiphilic polymer shell, i.e. having a hydrophilic portion, e.g., PEG, and a hydrophobic portion, e.g., PLA or 16 Appeal 2016-008166 Application 12/098,354 PLGA.” (Ans. 23.) Appellants have not disputed this finding. (See Reply Br. 11-18.) Therefore, we affirm the rejection of claims 1, 7, 8, 48, and 82—84 under 35 U.S.C. § 103(a) based on Farokhzad, Lanza, and Ruoslahti. Claims 2, 4, 15, 16, 20-22, 24, 25, and 63 have not been argued separately and fall with claim 1. 37 C.F.R. § 41.37(c)(l)(iv). Ill The Examiner has rejected claims 46-48 under 35 U.S.C. § 103(a) as obvious based on Farokhzad, Lanza, Ruoslahti, and Hoarau. We adopt the Examiner’s findings of fact and reasoning. (See Final Action 27—28.) Appellants argue that “Hoarau does not cure the deficiencies of Farokhzad, Lanza and Ruoslahti.” (Reply Br. 18.) However, for the reasons discussed above, we conclude that Farokhzad, Lanza and Ruoslahti support the Examiner’s rejection. We therefore affirm the rejection of claims 46-48 under 35 U.S.C. § 103(a) as obvious based on Farokhzad, Lanza, Ruoslahti, and Hoarau. IV The Examiner has rejected claims 25, 28, and 83 under 35 U.S.C. § 103(a) as obvious based on Farokhzad, Lanza, Ruoslahti, and Duncanson. The Examiner finds that, although “Farokhzad, Lanza and Ruoslahti do not expressly teach wherein the nanoparticle polymeric matrix comprises a lipid terminated PEG,” “Duncanson teaches polymeric target specific nanoparticles comprising . . . PLGA . . . and wherein the polymeric matrix comprises lipid terminated PEG.” (Final Action 29.) The Examiner 17 Appeal 2016-008166 Application 12/098,354 concludes that it would have been obvious to modify the nanoparticles made obvious by Farokhzad, Lanza, and Ruoslahti to use a polymer matrix comprising PLGA and lipid-terminated PEG because “lipid terminated PEG was an art recognized equivalent to the surfactants in the nanoparticles of Farokhzad. Moreover, lipid terminated PEG was effective for linking the targeting agent to the nanoparticle and was effective for reducing clearance of the nanoparticles via the reticuloendothelial system.” (Id.) We agree with the Examiner that the cited references would have made obvious the invention of claim 25, which is directed to the formulation of claim 1, where the nanoparticles comprise a copolymer of PLGA (polylactic-co-glycolic acid) and polyethylene glycol (PEG). The teachings of Farokhzad, Lanza, and Ruoslahti are discussed above. Duncanson discloses “polymeric particles comprised of poly(lactic acid) (PLA) with incorporated polyethylene glycol)-lipids (PEG-lipids).” (Duncanson 4991, abstract.) Duncanson states that “rapid clearance of particles to the reticuloendothelial system (RES) prevents delivery vehicles from reaching their designated target site” and “the most effective mitigation of RES- mediated particle clearance has been accomplished by surface grafting PEG to build a sterically repulsive shield that protects the particle from recognition by the RES.” (Id. at 4992, left col.) Duncanson also states that “a number of groups have incorporated a PEG copolymer in situ during particle formation. In this process a synthesized diblock copolymer such as PEG-PLA, PEG-PLGA, or a triblock copolymer such as PLA-PEG-PLA is directly incorporated.” (Id., citations omitted.) Duncanson discloses that 18 Appeal 2016-008166 Application 12/098,354 “the addition of PEG-lipids lead to a stable emulsion and an easily suspended final product. ... In contrast to conventionally used detergents, good biocompatibility and low toxicity of PEG-based lipopolymers is well documented in the literature.” {Id. at 4994, left col.) Thus, it would have been obvious to modify the nanoparticles made obvious by Farokhzad, Lanza, and Ruoslahti to use a polymer matrix comprising PLGA and lipid-terminated PEG because Duncanson teaches that PEG-PLGA had been used for such particles by others, and also teaches that lipid-terminated PEG leads to a stable emulsion, and has good biocompatibility and low toxicity. Appellants argue that Duncanson does not teach “selecting a ratio of functionalized to non-functionalized polymer (claim 83) nor lipid-terminated PEG (claim 28).” (Appeal Br. 32.) This argument is unpersuasive because, as discussed above, Duncanson provides sufficient reason for a person of ordinary skill in the art to use lipid-terminated PEG in the nanoparticles made obvious by the other cited references. In addition, claim 83 does not require any particular ratio of functionalized to non-functionalized polymer. We therefore affirm the rejection of claims 25, 28, and 83 under 35 U.S.C. § 103(a) based on based on Farokhzad, Lanza, Ruoslahti, and Duncanson. V The Examiner has rejected claim 13 as obvious based on Farokhzad, Lanza, Ruoslahti, and Chhatwal. Appellants have waived arguments based on Chhatwal. {See Appeal Br. 33.) We therefore affirm the rejection of claim 13 under 35 U.S.C. § 103(a) based on Farokhzad, Lanza, Ruoslahti, 19 Appeal 2016-008166 Application 12/098,354 and Chhatwal. See 37 C.F.R. § 41.37(c)(l)(iv) (Appeal Brief must contain “[t]he arguments of appellant with respect to each ground of rejection, and the basis therefor.”); Hyatt v. Dudas, 551 F.3d 1307, 1314 (Fed. Cir. 2008). SUMMARY We affirm all of the rejections on appeal. TIME PERIOD FOR RESPONSE No time period for taking any subsequent action in connection with this appeal may be extended under 37 C.F.R. § 1.136(a). AFFIRMED 20