Selection and analysis of anti‐cancer antibodies for cancer therapy obtained from antibody phage library

Kurosawa, Gene; Sumitomo, Mariko; Ukai, Yojiro; Subere, Juvy; Muramatsu, Chiho; Eguchi, Kaoru; Tanaka-Hashiba, Miho; Sugiura, M.; Ando, Moriyasu; Sato, Noriko; Inaba, Kazuki; Morigaki, Satoko; Takasaki, Akihiko; Akahori, Yasushi; Miyakawa, Shuichi; Uyama, Ichiro; Maeda, Koutarou; Shiroki, Ryoichi; Hoshinaga, Kiyotaka; Mizoguchi, Yoshikazu; Hattori, Yoshinobu; Sugioka, Atsushi; Kurosawa, Yoshikazu

doi:10.1111/j.1349-7006.2010.01739.x

Cited by 17 publications

(18 citation statements)

References 22 publications

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“…Recent interest has focused on designing unbiased phenotypic screens wherein the identification of function-blocking effects precede efforts to dissect the underlying molecular mechanisms that give rise to the desired outcomes (13,15,31,32). With increasing evidence that cell behavior in 3D culture systems more faithfully recapitulates in vivo function, greater emphasis has been placed on developing improved in vitro models for screening purposes, including the use of basement membranelike gels, pepsin extracts of dermal collagen, and synthetic hydrogels (1, 2, 6, 33-35).…”

Section: Discussionmentioning

confidence: 99%

A 3D matrix platform for the rapid generation of therapeutic anti-human carcinoma monoclonal antibodies

Dudley¹,

Li²,

Hu³

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

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Efforts to develop unbiased screens for identifying novel functionblocking monoclonal antibodies (mAbs) in human carcinomatous states have been hampered by the limited ability to design in vitro models that recapitulate tumor cell behavior in vivo. Given that only invasive carcinoma cells gain permanent access to type I collagen-rich interstitial tissues, an experimental platform was established in which human breast cancer cells were embedded in 3D aldimine cross-linked collagen matrices and used as an immunogen to generate mAb libraries. In turn, cancer-cell-reactive antibodies were screened for their ability to block carcinoma cell proliferation within collagen hydrogels that mimic the in vivo environment. As a proof of principle, a single function-blocking mAb out of 15 identified was selected for further analysis and found to be capable of halting carcinoma cell proliferation, inducing apoptosis, and exerting global changes in gene expression in vitro. The ability of this mAb to block carcinoma cell proliferation and metastatic activity was confirmed in vivo, and the target antigen was identified by mass spectroscopy as the α 2 subunit of the α 2 β 1 integrin, one of the major type I collagen-binding receptors in mammalian cells. Validating the ability of the in vitro model to predict patterns of antigen expression in the disease setting, immunohistochemical analyses of tissues from patients with breast cancer verified markedly increased expression of the α 2 subunit in vivo. These results not only highlight the utility of this discovery platform for rapidly selecting and characterizing function-blocking, anticancer mAbs in an unbiased fashion, but also identify α 2 β 1 as a potential target in human carcinomatous states.n mammalian systems, a specialized form of extracellular matrix (ECM), termed the basement membrane, normally separates epithelial cells from the underlying type I collagen-rich interstitial matrix (1, 2). Thus, in mature animals and under physiologic conditions, the epithelium does not establish stable physical contacts with interstitial tissues (1, 2). In contrast, in neoplastic states, transformed epithelial cells (i.e., carcinomas) dissolve the intervening basement membrane barrier and establish adhesive interactions with the newly exposed type I collagen fibrillar network (1-5). As carcinoma cells begin to infiltrate the interstitial matrix, they rapidly adapt themselves to their 3D environment and initiate the proliferative phenotypes that define tumor progression at both primary and metastatic sites (2, 6, 7). Indeed, emphasizing the importance of the tumor-ECM interface, carcinoma cells do not simply use the surrounding interstitial matrix as a passive substrate, but actively promote increased type I collagen deposition within the peritumoral microenvironment as a means of further enhancing invasive activity, local growth, and cancer stem cell formation (7-12).Despite the importance of the carcinoma cell-type I collagen interface in vivo, therapeutic interventions that directly inte...

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Section: Discussionmentioning

confidence: 99%

A 3D matrix platform for the rapid generation of therapeutic anti-human carcinoma monoclonal antibodies

Dudley¹,

Li²,

Hu³

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

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“…However, the composition of the cell surface is very complex, with many types of proteins, carbohydrates and lipids, but with a low number of tumor-specific antigens. Non-specific adhesion and loss of specific ligand are among the problems often faced when intact cancer cells are used as the target to screen an antibody library (15). Under these conditions, an antibody library of high diversity and library size is particularly important.…”

Section: Discussionmentioning

confidence: 99%

Screening for antibodies against intact cancer cells with a naï¿½ve large phage antibody library

Zhou²,

Wang³

et al. 2011

Int J Mol Med

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Abstract. Large phage antibody libraries are expected to be an efficient technology for obtaining humanized anti-tumor antibodies. However, few reports have been concerned about the selection strategies for intact cancer cells as targets. In this study, a 2x1011 large naïve scFv library from blood B lymphocytes of normal adult donors and neonatal cord blood was constructed using the LoxP-cre system. Three human esophageal cancer cell lines were equally mixed for use as the target. These intact cells were divided into two groups, PF and NF, according to the treatment method of the cells (fixed with 2% PFA or not, respectively). Positive phage antibodies were identified following 4 panning cycles of adhesion, elution and amplification. Using a cell ELISA assay, it was found that the additional procedure of directly infecting XL1-Blue bacteria with the cell pellet following washing with an acidic solution can effectively decrease the loss of positive phage, yielding a positive screening rate of 11.6% (61/525). Most of the phage antibodies displayed binding activity with all three esophageal cancer cell lines. Moreover, other phages (such as NFc53a and NFc70a) appeared to be specific for certain cell lines. Regarding the method used to treat the target cells, both the positive screening rate and the genetic diversity of the antibody variable region were significantly higher in the NF group (12.9 and 71.4%, respectively) than in the PF group (10.5 and 14.2%, respectively). Immunohistochemical analysis demonstrated that the scFv phages have good specificity for esophageal cancer. This technology is helpful for developing small molecular tracers and targeted therapies for malignant tumors.

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“…To date, most antibodies identified by phenotypic screens have been found using a two-step process. First, antibody populations have been enriched against a target cell or tissue type before being screened for function [11][12][13][14][15][16][17][18]. A two-step process is dependent on the efficiency of both steps; however, the functional screen poses the greatest challenge and is often the bottleneck in the process.…”

Section: Phenotypic Screening Of Human B Cell Repertoiresmentioning

confidence: 99%

“…There have been several successful phenotypic screens, performed on these enriched populations, which have generated antibodies against cancer cells and infectious agents. As early as 1995, de Kruif et al [11] screened for target cell specificity and more recent examples have followed [12][13][14]. Functional screens have also been performed that have identified antibodies that induce apoptosis [15], inhibit cell proliferation [16], or internalise [17,18].…”

mentioning

confidence: 99%

Phenotypic screening: the future of antibody discovery

González-Muñoz

Minter

Rust

2016

Drug Discovery Today

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Selection and analysis of anti‐cancer antibodies for cancer therapy obtained from antibody phage library

Cited by 17 publications

References 22 publications

A 3D matrix platform for the rapid generation of therapeutic anti-human carcinoma monoclonal antibodies

A 3D matrix platform for the rapid generation of therapeutic anti-human carcinoma monoclonal antibodies

Screening for antibodies against intact cancer cells with a naï¿½ve large phage antibody library

Phenotypic screening: the future of antibody discovery

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