Construction of in vitro 3-D model for lung cancer-cell metastasis study

Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interac...

Full description

Saved in:

Bibliographic Details
Published in:	BMC cancer Vol. 22; no. 1; pp. 438 - 9
Main Authors:	Jiang, Rongrong, Huang, Jiechun, Sun, Xiaotian, Chu, Xianglin, Wang, Fangrui, Zhou, Jie, Fan, Qihui, Pang, Liewen
Format:	Journal Article
Language:	English
Published:	London BioMed Central 21.04.2022 BioMed Central Ltd Springer Nature B.V BMC
Subjects:	3-D model Alveoli Animal models Animals Biomedical and Life Sciences Biomedicine Cancer Cancer metastasis Cancer Research Care and treatment Cell adhesion & migration Cell culture Cell morphology Cell proliferation Collagen Collagen - metabolism Collagen hydrogel Complications and side effects Cytology Diagnosis Drug delivery Drug screening Epithelial cells Etching Extracellular matrix Extracellular Matrix - metabolism Health Promotion and Disease Prevention Humans Hydrogels Hydrogels - analysis Hydrogels - chemistry Hydrogels - metabolism Immunosuppressive agents Lung cancer Lung Neoplasms - metabolism Medicine/Public Health Mesenchyme Metastases Metastasis Microfluidic system Microfluidics Mimicry Morphology Neoplasm Invasiveness Oncology Oncology, Experimental Penicillin Porous materials Silicon wafers Surgical Oncology Tumor cells Tumor Microenvironment China Cancer metastasis Collagen hydrogel Drug screening Microfluidic system 3-D model
ISSN:	1471-2407, 1471-2407
Online Access:	Get full text
Tags:	Add Tag No Tags, Be the first to tag this record!

Abstract	Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests. Methods Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo . Results A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers. Conclusions A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo .
AbstractList	Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests. Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo. A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers. A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo. Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests. Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo. A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo. Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests. Methods Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo. Results A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers. Conclusions A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo. Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests. Methods Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo . Results A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers. Conclusions A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo . Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests. Methods Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo. Results A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers. Conclusions A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo. Keywords: 3-D model, Collagen hydrogel, Cancer metastasis, Drug screening, Microfluidic system Abstract Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests. Methods Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo. Results A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers. Conclusions A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo. Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests.BACKGROUNDCancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially due to the short of effective in vitro model for cell invasion studies. The traditional 2-D culture method cannot reveal the interaction between cells and the surrounding extracellular matrix during invasion process, while the animal models usually are too complex to explain mechanisms in detail. Therefore, a precise and efficient 3-D in vitro model is highly desirable for cell invasion studies and drug screening tests.Precise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo.METHODSPrecise micro-fabrication techniques are developed and integrated with soft hydrogels for constructing of 3-D lung-cancer micro-environment, mimicking the pulmonary gland or alveoli as in vivo.A 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers.RESULTSA 3-D in vitro model for cancer cell culture and metastasis studies is developed with advanced micro-fabrication technique, combining microfluidic system with soft hydrogel. The constructed microfluidic platform can provide nutrition and bio-chemical factors in a continuous transportation mode and has the potential to form stable chemical gradient for cancer invasion research. Hundreds of micro-chamber arrays are constructed within the collagen gel, ensuring that all surrounding substrates for tumor cells are composed of natural collagen hydrogel, like the in vivo micro-environment. The 3-D in vitro model can also provide a fully transparent platform for the visual observation of the cell morphology, proliferation, invasion, cell-assembly, and even the protein expression by immune-fluorescent tests if needed. The lung-cancer cells A549 and normal lung epithelial cells (HPAEpiCs) have been seeded into the 3-D system. It is found out that cells can normally proliferate in the microwells for a long period. Moreover, although the cancer cells A549 and alveolar epithelial cells HPAEpiCs have the similar morphology on 2-D solid substrate, in the 3-D system the cancer cells A549 distributed sparsely as single round cells on the extracellular matrix (ECM) when they attached to the substrate, while the normal lung epithelial cells can form cell aggregates, like the structure of normal tissue. Importantly, cancer cells cultured in the 3-D in vitro model can exhibit the interaction between cells and extracellular matrix. As shown in the confocal microscope images, the A549 cells present round and isolated morphology without much invasion into ECM, while starting from around Day 5, cells changed their shape to be spindle-like, as in mesenchymal morphology, and then started to destroy the surrounding ECM and invade out of the micro-chambers.A 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo.CONCLUSIONSA 3-D in vitro model is constructed for cancer cell invasion studies, combining the microfluidic system and micro-chamber structures within hydrogel. To show the invasion process of lung cancer cells, the cell morphology, proliferation, and invasion process are all analyzed. The results confirmed that the micro-environment in the 3-D model is vital for revealing the lung cancer cell invasion as in vivo.
ArticleNumber	438
Audience	Academic
Author	Jiang, Rongrong Zhou, Jie Wang, Fangrui Pang, Liewen Fan, Qihui Huang, Jiechun Sun, Xiaotian Chu, Xianglin
Author_xml	– sequence: 1 givenname: Rongrong surname: Jiang fullname: Jiang, Rongrong organization: Department of Cardiothoracic Surgery, Huashan Hospital, Fudan University – sequence: 2 givenname: Jiechun surname: Huang fullname: Huang, Jiechun organization: Department of Cardiothoracic Surgery, Huashan Hospital, Fudan University – sequence: 3 givenname: Xiaotian surname: Sun fullname: Sun, Xiaotian organization: Department of Cardiothoracic Surgery, Huashan Hospital, Fudan University – sequence: 4 givenname: Xianglin surname: Chu fullname: Chu, Xianglin organization: Department of Cardiothoracic Surgery, Huashan Hospital, Fudan University – sequence: 5 givenname: Fangrui surname: Wang fullname: Wang, Fangrui organization: Department of Cardiothoracic Surgery, Huashan Hospital, Fudan University – sequence: 6 givenname: Jie surname: Zhou fullname: Zhou, Jie organization: Qibao Community Health Service Center – sequence: 7 givenname: Qihui surname: Fan fullname: Fan, Qihui email: fanqh@iphy.ac.cn organization: Beijing National Laboratory for Condensed Matter Physics and Laboratory of Soft Matter and Biological Physics, Institute of Physics, Chinese Academy of Sciences – sequence: 8 givenname: Liewen surname: Pang fullname: Pang, Liewen email: plwmd1967@126.com organization: Department of Cardiothoracic Surgery, Huashan Hospital, Fudan University
BackLink	https://www.ncbi.nlm.nih.gov/pubmed/35449036$$D View this record in MEDLINE/PubMed
BookMark	eNp9kklr3DAAhU1JaZb2D_RQDIXSHpxql3UJhOmSgUChy1loZMmjwSOlkhyaf185kzTjUGIbZOTvPUnP77g68MGbqnoNwSmELfuYIGpb2gCEGiAoYY14Vh1BwmGDCOAHe--H1XFKGwAgb0H7ojrElBABMDuqLhbBpxxHnV3wdbC18_W1yzHUuPlUb0NnhtqGWA-j72utvDax0WYY6q3JKpXHpTrlsbt5WT23akjm1d14Uv368vnn4qK5_PZ1uTi_bDTjKDe6VasOUsO5sFgzhpWwwFpCOAJUEQwRZIwzqAUGghNMBbHadB2maNVZRPFJtdz5dkFt5FV0WxVvZFBO3k6E2EsVs9ODkXClLeBEQKZaYjtWFmZwRa1AHVSMsuJ1tvO6Gldb02njc1TDzHT-xbu17MO1FADxFpNi8P7OIIbfo0lZbl2a4lHehDFJxCgp_wgX-KR6-wjdhDH6ElWhygW4YOKB6lU5gPM2lHX1ZCrPOYAYUQJBoU7_Q5W7M1unS0msK_MzwYeZoDDZ_Mm9GlOSyx_f5-y7PXZt1JDXKQzjVJA0B9_sp_cvtvtyFaDdATqGlKKxUrusJp-yXTdICOTUY7nrsSw9lrc9llMO6JH03v1JEd6JUoF9b-JDxE-o_gLj2P_m
CitedBy_id	crossref_primary_10_1165_rcmb_2024_0479ST crossref_primary_10_1146_annurev_bioeng_110222_102142 crossref_primary_10_3390_ijms23137444 crossref_primary_10_1186_s12929_024_00994_y crossref_primary_10_1016_j_bbcan_2025_189293 crossref_primary_10_1016_j_mtbio_2025_102130 crossref_primary_10_1016_j_adcanc_2022_100076 crossref_primary_10_3390_ijms241914516 crossref_primary_10_12677_wjcr_2025_153014
Cites_doi	10.1039/C7LC00191F 10.1016/j.biomaterials.2015.02.022 10.1111/joim.13201 10.1016/j.biotechadv.2014.07.009 10.1073/pnas.1212834109 10.1016/j.biomaterials.2010.04.064 10.1039/c000022a 10.1016/j.mattod.2015.05.002 10.1126/scitranslmed.3009367 10.1002/1097-0282(200009)54:3<222::AID-BIP80>3.0.CO;2-K 10.1038/nrc2544 10.1016/j.addr.2014.06.002 10.1038/nmat2619 10.1038/s41568-018-0104-6 10.1073/pnas.1102808108 10.1038/nrc3080 10.1039/c2lc21202a 10.1007/s10555-016-9618-0 10.18632/oncotarget.5874 10.1038/s41598-018-36347-7 10.1016/j.biomaterials.2007.12.044 10.3389/fcell.2015.00004 10.1063/1.4979104 10.1126/sciadv.aat5847 10.1038/nature14377 10.18632/oncotarget.8232 10.1016/j.cell.2013.11.029 10.1038/s41598-018-30683-4
ContentType	Journal Article
Copyright	The Author(s) 2022 2022. The Author(s). COPYRIGHT 2022 BioMed Central Ltd. 2022. This work is licensed under http://creativecommons.org/licenses/by/4.0/ (the “License”). Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.
Copyright_xml	– notice: The Author(s) 2022 – notice: 2022. The Author(s). – notice: COPYRIGHT 2022 BioMed Central Ltd. – notice: 2022. This work is licensed under http://creativecommons.org/licenses/by/4.0/ (the “License”). Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.
DBID	C6C AAYXX CITATION CGR CUY CVF ECM EIF NPM ISR 3V. 7TO 7X7 7XB 88E 8FI 8FJ 8FK ABUWG AFKRA AZQEC BENPR CCPQU DWQXO FYUFA GHDGH H94 K9. M0S M1P PHGZM PHGZT PIMPY PJZUB PKEHL PPXIY PQEST PQQKQ PQUKI PRINS 7X8 5PM DOA
DOI	10.1186/s12885-022-09546-9
DatabaseName	Springer Nature OA Free Journals CrossRef Medline MEDLINE MEDLINE (Ovid) MEDLINE MEDLINE PubMed Gale In Context: Science ProQuest Central (Corporate) Oncogenes and Growth Factors Abstracts Health & Medical Collection ProQuest Central (purchase pre-March 2016) Medical Database (Alumni Edition) Hospital Premium Collection Hospital Premium Collection (Alumni Edition) ProQuest Central (Alumni) (purchase pre-March 2016) ProQuest Central (Alumni) ProQuest Central UK/Ireland ProQuest Central Essentials ProQuest Central ProQuest One Community College ProQuest Central Health Research Premium Collection Health Research Premium Collection (Alumni) AIDS and Cancer Research Abstracts ProQuest Health & Medical Complete (Alumni) ProQuest Health & Medical Collection Medical Database ProQuest Central Premium ProQuest One Academic Publicly Available Content Database ProQuest Health & Medical Research Collection ProQuest One Academic Middle East (New) One Health & Nursing ProQuest One Academic Eastern Edition (DO NOT USE) ProQuest One Academic (retired) ProQuest One Academic UKI Edition ProQuest Central China MEDLINE - Academic PubMed Central (Full Participant titles) DOAJ Directory of Open Access Journals
DatabaseTitle	CrossRef MEDLINE Medline Complete MEDLINE with Full Text PubMed MEDLINE (Ovid) Publicly Available Content Database Oncogenes and Growth Factors Abstracts ProQuest One Academic Middle East (New) ProQuest Central Essentials ProQuest Health & Medical Complete (Alumni) ProQuest Central (Alumni Edition) ProQuest One Community College ProQuest One Health & Nursing ProQuest Central China ProQuest Central ProQuest Health & Medical Research Collection Health Research Premium Collection Health and Medicine Complete (Alumni Edition) ProQuest Central Korea Health & Medical Research Collection AIDS and Cancer Research Abstracts ProQuest Central (New) ProQuest Medical Library (Alumni) ProQuest One Academic Eastern Edition ProQuest Hospital Collection Health Research Premium Collection (Alumni) ProQuest Hospital Collection (Alumni) ProQuest Health & Medical Complete ProQuest Medical Library ProQuest One Academic UKI Edition ProQuest One Academic ProQuest One Academic (New) ProQuest Central (Alumni) MEDLINE - Academic
DatabaseTitleList	MEDLINE Publicly Available Content Database MEDLINE - Academic
Database_xml	– sequence: 1 dbid: DOA name: DOAJ Directory of Open Access Journals url: https://www.doaj.org/ sourceTypes: Open Website – sequence: 2 dbid: NPM name: PubMed url: http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed sourceTypes: Index Database – sequence: 3 dbid: PIMPY name: Publicly Available Content Database url: http://search.proquest.com/publiccontent sourceTypes: Aggregation Database
DeliveryMethod	fulltext_linktorsrc
Discipline	Medicine
EISSN	1471-2407
EndPage	9
ExternalDocumentID	oai_doaj_org_article_1bcf074916a84fd6bd161b5f92d1a656 PMC9027834 A701325410 35449036 10_1186_s12885_022_09546_9
Genre	Journal Article
GeographicLocations	China
GeographicLocations_xml	– name: China
GroupedDBID	--- 0R~ 23N 2WC 53G 5VS 6J9 6PF 7X7 88E 8FI 8FJ AAFWJ AAJSJ AASML AAWTL ABDBF ABUWG ACGFO ACGFS ACIHN ACMJI ACPRK ACUHS ADBBV ADRAZ ADUKV AEAQA AENEX AFKRA AFPKN AHBYD AHMBA AHYZX ALMA_UNASSIGNED_HOLDINGS AMKLP AMTXH AOIJS BAPOH BAWUL BCNDV BENPR BFQNJ BMC BPHCQ BVXVI C6C CCPQU CS3 DIK DU5 E3Z EAD EAP EAS EBD EBLON EBS EMB EMK EMOBN ESX F5P FYUFA GROUPED_DOAJ GX1 HMCUK HYE IAO IHR IHW INH INR ISR ITC KQ8 M1P M48 M~E O5R O5S OK1 OVT P2P PGMZT PHGZM PHGZT PIMPY PJZUB PPXIY PQQKQ PROAC PSQYO PUEGO RBZ RNS ROL RPM RSV SBL SOJ SV3 TR2 TUS U2A UKHRP W2D WOQ WOW XSB AAYXX AFFHD CITATION -A0 3V. ACRMQ ADINQ ALIPV C24 CGR CUY CVF ECM EIF NPM 7TO 7XB 8FK AZQEC DWQXO H94 K9. PKEHL PQEST PQUKI PRINS 7X8 5PM
ID	FETCH-LOGICAL-c672t-c8abd15e779f3c663a9f0ff447205a4312166761c9309743594fcedd352bdf253
IEDL.DBID	RSV
ISICitedReferencesCount	11
ISICitedReferencesURI	http://www.webofscience.com/api/gateway?GWVersion=2&SrcApp=Summon&SrcAuth=ProQuest&DestLinkType=CitingArticles&DestApp=WOS_CPL&KeyUT=000784612600001&url=https%3A%2F%2Fcvtisr.summon.serialssolutions.com%2F%23%21%2Fsearch%3Fho%3Df%26include.ft.matches%3Dt%26l%3Dnull%26q%3D
ISSN	1471-2407
IngestDate	Fri Oct 03 12:43:31 EDT 2025 Tue Nov 04 02:00:55 EST 2025 Sun Nov 09 14:03:21 EST 2025 Mon Oct 06 18:34:27 EDT 2025 Tue Nov 11 10:39:29 EST 2025 Tue Nov 04 18:06:08 EST 2025 Thu Nov 13 14:23:31 EST 2025 Thu May 22 21:22:24 EDT 2025 Thu Jan 02 22:55:52 EST 2025 Sat Nov 29 06:42:34 EST 2025 Tue Nov 18 22:08:59 EST 2025 Sat Sep 06 07:18:37 EDT 2025
IsDoiOpenAccess	true
IsOpenAccess	true
IsPeerReviewed	true
IsScholarly	true
Issue	1
Keywords	Cancer metastasis Collagen hydrogel Drug screening Microfluidic system 3-D model
Language	English
License	2022. The Author(s). Open AccessThis article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons licence, and indicate if changes were made. The images or other third party material in this article are included in the article's Creative Commons licence, unless indicated otherwise in a credit line to the material. If material is not included in the article's Creative Commons licence and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this licence, visithttp://creativecommons.org/licenses/by/4.0/. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated in a credit line to the data.
LinkModel	DirectLink
MergedId	FETCHMERGED-LOGICAL-c672t-c8abd15e779f3c663a9f0ff447205a4312166761c9309743594fcedd352bdf253
Notes	ObjectType-Article-1 SourceType-Scholarly Journals-1 ObjectType-Feature-2 content type line 14 content type line 23
OpenAccessLink	https://link.springer.com/10.1186/s12885-022-09546-9
PMID	35449036
PQID	2666607969
PQPubID	44074
PageCount	9
ParticipantIDs	doaj_primary_oai_doaj_org_article_1bcf074916a84fd6bd161b5f92d1a656 pubmedcentral_primary_oai_pubmedcentral_nih_gov_9027834 proquest_miscellaneous_2654288378 proquest_journals_2666607969 gale_infotracmisc_A701325410 gale_infotracacademiconefile_A701325410 gale_incontextgauss_ISR_A701325410 gale_healthsolutions_A701325410 pubmed_primary_35449036 crossref_citationtrail_10_1186_s12885_022_09546_9 crossref_primary_10_1186_s12885_022_09546_9 springer_journals_10_1186_s12885_022_09546_9
PublicationCentury	2000
PublicationDate	2022-04-21
PublicationDateYYYYMMDD	2022-04-21
PublicationDate_xml	– month: 04 year: 2022 text: 2022-04-21 day: 21
PublicationDecade	2020
PublicationPlace	London
PublicationPlace_xml	– name: London – name: England
PublicationTitle	BMC cancer
PublicationTitleAbbrev	BMC Cancer
PublicationTitleAlternate	BMC Cancer
PublicationYear	2022
Publisher	BioMed Central BioMed Central Ltd Springer Nature B.V BMC
Publisher_xml	– name: BioMed Central – name: BioMed Central Ltd – name: Springer Nature B.V – name: BMC
References	AM Jimenez Valencia (9546_CR7) 2015; 6 W Asghar (9546_CR9) 2015; 18 T Yu (9546_CR17) 2016; 7 AO Brightman (9546_CR26) 2000; 54 LY Liu (9546_CR12) 2011; 108 KV Nguyen-Ngoc (9546_CR5) 2012; 109 HH Song (9546_CR23) 2014; 79–80 J Sainz de Aja (9546_CR27) 2021; 289 A Jacob (9546_CR28) 2015; 3 DW Hutmacher (9546_CR25) 2010; 9 DT Butcher (9546_CR15) 2009; 9 HH Popper (9546_CR4) 2016; 35 A Sontheimer-Phelps (9546_CR14) 2019; 19 KJ Cheung (9546_CR3) 2013; 155 MM Shen (9546_CR2) 2015; 520 QH Fan (9546_CR20) 2017; 17 TJ Liu (9546_CR24) 2010; 10 J Sapudom (9546_CR6) 2015; 52 M Miron-Mendoza (9546_CR13) 2010; 31 T Osaki (9546_CR19) 2018; 4 J Plou (9546_CR18) 2018; 8 D Wirtz (9546_CR8) 2011; 11 K Tanner (9546_CR1) 2015; 7 X Xu (9546_CR10) 2014; 32 AP Wong (9546_CR22) 2008; 29 J Kim (9546_CR11) 2012; 12 W Diao (9546_CR21) 2019; 9 A Zuchowska (9546_CR16) 2017; 11
References_xml	– volume: 17 start-page: 2852 issue: 16 year: 2017 ident: 9546_CR20 publication-title: Lab Chip doi: 10.1039/C7LC00191F – volume: 52 start-page: 367 year: 2015 ident: 9546_CR6 publication-title: Biomaterials doi: 10.1016/j.biomaterials.2015.02.022 – volume: 289 start-page: 629 issue: 5 year: 2021 ident: 9546_CR27 publication-title: J Intern Med doi: 10.1111/joim.13201 – volume: 32 start-page: 1256 issue: 7 year: 2014 ident: 9546_CR10 publication-title: Biotechnol Adv doi: 10.1016/j.biotechadv.2014.07.009 – volume: 109 start-page: E2595 issue: 39 year: 2012 ident: 9546_CR5 publication-title: Proc Natl Acad Sci USA doi: 10.1073/pnas.1212834109 – volume: 31 start-page: 6425 issue: 25 year: 2010 ident: 9546_CR13 publication-title: Biomaterials doi: 10.1016/j.biomaterials.2010.04.064 – volume: 10 start-page: 1671 issue: 13 year: 2010 ident: 9546_CR24 publication-title: Lab Chip doi: 10.1039/c000022a – volume: 18 start-page: 539 issue: 10 year: 2015 ident: 9546_CR9 publication-title: Mater Today doi: 10.1016/j.mattod.2015.05.002 – volume: 7 start-page: 283ps9 issue: 283 year: 2015 ident: 9546_CR1 publication-title: Sci Transl Med doi: 10.1126/scitranslmed.3009367 – volume: 54 start-page: 222 issue: 3 year: 2000 ident: 9546_CR26 publication-title: Biopolymers doi: 10.1002/1097-0282(200009)54:3<222::AID-BIP80>3.0.CO;2-K – volume: 9 start-page: 108 issue: 2 year: 2009 ident: 9546_CR15 publication-title: Nat Rev Cancer doi: 10.1038/nrc2544 – volume: 79–80 start-page: 19 year: 2014 ident: 9546_CR23 publication-title: Adv Drug Deliv Rev doi: 10.1016/j.addr.2014.06.002 – volume: 9 start-page: 90 issue: 2 year: 2010 ident: 9546_CR25 publication-title: Nat Mater doi: 10.1038/nmat2619 – volume: 19 start-page: 65 issue: 2 year: 2019 ident: 9546_CR14 publication-title: Nat Rev Cancer doi: 10.1038/s41568-018-0104-6 – volume: 108 start-page: 6853 issue: 17 year: 2011 ident: 9546_CR12 publication-title: Proc Natl Acad Sci USA doi: 10.1073/pnas.1102808108 – volume: 11 start-page: 512 issue: 7 year: 2011 ident: 9546_CR8 publication-title: Nat Rev Cancer doi: 10.1038/nrc3080 – volume: 12 start-page: 1813 issue: 10 year: 2012 ident: 9546_CR11 publication-title: Lab Chip doi: 10.1039/c2lc21202a – volume: 35 start-page: 75 issue: 1 year: 2016 ident: 9546_CR4 publication-title: Cancer Metastasis Rev doi: 10.1007/s10555-016-9618-0 – volume: 6 start-page: 43438 issue: 41 year: 2015 ident: 9546_CR7 publication-title: Oncotarget doi: 10.18632/oncotarget.5874 – volume: 9 start-page: 85 issue: 1 year: 2019 ident: 9546_CR21 publication-title: Sci Rep doi: 10.1038/s41598-018-36347-7 – volume: 29 start-page: 1853 issue: 12 year: 2008 ident: 9546_CR22 publication-title: Biomaterials doi: 10.1016/j.biomaterials.2007.12.044 – volume: 3 start-page: 4 year: 2015 ident: 9546_CR28 publication-title: Front Cell Dev Biol doi: 10.3389/fcell.2015.00004 – volume: 11 start-page: 024110 issue: 2 year: 2017 ident: 9546_CR16 publication-title: Biomicrofluidics doi: 10.1063/1.4979104 – volume: 4 start-page: eaat5847 issue: 10 year: 2018 ident: 9546_CR19 publication-title: Sci Adv doi: 10.1126/sciadv.aat5847 – volume: 520 start-page: 298 issue: 7547 year: 2015 ident: 9546_CR2 publication-title: Nature doi: 10.1038/nature14377 – volume: 7 start-page: 25593 issue: 18 year: 2016 ident: 9546_CR17 publication-title: Oncotarget doi: 10.18632/oncotarget.8232 – volume: 155 start-page: 1639 issue: 7 year: 2013 ident: 9546_CR3 publication-title: Cell doi: 10.1016/j.cell.2013.11.029 – volume: 8 start-page: 12723 issue: 1 year: 2018 ident: 9546_CR18 publication-title: Sci Rep doi: 10.1038/s41598-018-30683-4
SSID	ssj0017808
Score	2.4114213
Snippet	Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is... Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is partially... Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking, which is... Abstract Background Cancer metastasis is the main cause of mortality in cancer patients. However, the drugs targeting metastasis processes are still lacking,...
SourceID	doaj pubmedcentral proquest gale pubmed crossref springer
SourceType	Open Website Open Access Repository Aggregation Database Index Database Enrichment Source Publisher
StartPage	438
SubjectTerms	3-D model Alveoli Animal models Animals Biomedical and Life Sciences Biomedicine Cancer Cancer metastasis Cancer Research Care and treatment Cell adhesion & migration Cell culture Cell morphology Cell proliferation Collagen Collagen - metabolism Collagen hydrogel Complications and side effects Cytology Diagnosis Drug delivery Drug screening Epithelial cells Etching Extracellular matrix Extracellular Matrix - metabolism Health Promotion and Disease Prevention Humans Hydrogels Hydrogels - analysis Hydrogels - chemistry Hydrogels - metabolism Immunosuppressive agents Lung cancer Lung Neoplasms - metabolism Medicine/Public Health Mesenchyme Metastases Metastasis Microfluidic system Microfluidics Mimicry Morphology Neoplasm Invasiveness Oncology Oncology, Experimental Penicillin Porous materials Silicon wafers Surgical Oncology Tumor cells Tumor Microenvironment
SummonAdditionalLinks	– databaseName: DOAJ Directory of Open Access Journals dbid: DOA link: http://cvtisr.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwrV1Jb9YwELVQhRAXxE6ggEFIHMBqEu_HslTlQIVYpN4sxwtEKgn68rW_n7Gz0BQBFy45xBMpmcXzJrbfIPRMllIG2nhSMmcJ43BpBG1IiE64BiroyvvcbEIeHanjY_3hXKuvtCdspAceFbdXNS5CmgMUYxWLXjQeMErDo659ZQGMpNkXUM9cTE3rB1KVaj4io8TeALOwSieRawKQggmiV2kos_X_PiefS0oXN0xeWDXNyejgOro2oUi8P779DXQpdDfRlffTOvktdJj6cM7MsLiPuO3wWbvd9JiSNzh3v8GAVvEJhDp2yfAbkn7h4-9hawEvDu2AM_HsbfTl4O3n14dk6plAnJD1ljhlQUM8SKkjdQAnrI5ljIzJuuQW0EJdpV2tldO0hFKCcs2iC94DDmt8rDm9g3a6vgv3EI7eSSsDVxFSWBW8heLMSqo8DaKGsq1A1axC4yZC8dTX4sTkwkIJM6rdgNpNVrvRBXqxPPNjpNP4q_SrZJlFMlFh5xvgIGZyEPMvBynQ42RXM54rXQLa7Mu0zMRZVRboaZZIdBhd2m_z1Z4Og3n36eNK6PkkFHv4Smen4wugq8SgtZLcXUlCvLr18OxgZpovBgMwSYhSagHf_GQZTk-mPXBd6E-TDGepN7RUBbo7-uOiGcoZ0wBGCiRXnrpS3Xqka79lNnFd5mYrBXo5-_Sv1_qzae7_D9M8QFfrHJOM1NUu2oG4CA_RZXe2bYfNoxzRPwFc2ErX priority: 102 providerName: Directory of Open Access Journals – databaseName: ProQuest Central dbid: BENPR link: http://cvtisr.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwpV1Lb9QwELZgixAX3o9AAYOQOIDVPBw_TqiFVuXAqiog9WY5fpSVSlI22_5-xl4nJUX0wmUP8URae17fZMYzCL3hOeeuaizJqdGE1vDTsKohzhtmGoigC2vjsAk-n4ujI3mQPrj1qaxysInRUNvOhG_kW-BIGMu5ZPLD6S8SpkaF7GoaoXEdbYROZXSGNnZ25weHYx6Bi1wMV2UE2-rBGotwI7kkAC0oI3LijmLX_r9t8x_O6XLh5KXsaXRKe3f-dzt30e0ER_H2Wn7uoWuuvY9ufkkJ9wdoPwz0HFrM4s7jRYvPF6tlhyvyCccxOhhgLz4Bm4FNkKAlCbkA_NOtNADPftHj2MH2Ifq-t_vt4z5JwxeIYbxcESN0Y4vacS59ZQCXaOlz7ynlZV5rgB1lEcpjCyOrHGKSqpbUG2ctALrG-rKuHqFZ27XuCcLeGq65q4UHX1g4qyHK07wStnKshPgvQ8XAA2VSZ_IwIONExQhFMLXmmwK-qcg3JTP0bnzndN2X40rqncDakTL01I4PuuWxSiqqisZ4AFSAl7Wg3jLYPiua2svSFhpgb4ZeBsFQ6wuqo2VQ2zzkq2pa5Bl6HSlCX402FO4c67O-V5-_Hk6I3iYi38EujU73IOCsQiuuCeXmhBIU30yXB9FSyfD06kKuMvRqXA5vhmK61nVngaamYcg0Fxl6vBbo8WSqmlIJqCZDfCLqk6ObrrSLH7Etuczj1JYMvR-U4uJv_Zs1T6_exTN0q4zqSklZbKIZSLx7jm6Y89WiX75I6v4bI2BaVg priority: 102 providerName: ProQuest
Title	Construction of in vitro 3-D model for lung cancer-cell metastasis study
URI	https://link.springer.com/article/10.1186/s12885-022-09546-9 https://www.ncbi.nlm.nih.gov/pubmed/35449036 https://www.proquest.com/docview/2666607969 https://www.proquest.com/docview/2654288378 https://pubmed.ncbi.nlm.nih.gov/PMC9027834 https://doaj.org/article/1bcf074916a84fd6bd161b5f92d1a656
Volume	22
WOSCitedRecordID	wos000784612600001&url=https%3A%2F%2Fcvtisr.summon.serialssolutions.com%2F%23%21%2Fsearch%3Fho%3Df%26include.ft.matches%3Dt%26l%3Dnull%26q%3D
hasFullText	1
inHoldings	1
isFullTextHit
isPrint
journalDatabaseRights	– providerCode: PRVADU databaseName: Open Access: BioMedCentral Open Access Titles customDbUrl: eissn: 1471-2407 dateEnd: 99991231 omitProxy: false ssIdentifier: ssj0017808 issn: 1471-2407 databaseCode: RBZ dateStart: 20010101 isFulltext: true titleUrlDefault: https://www.biomedcentral.com/search/ providerName: BioMedCentral – providerCode: PRVAON databaseName: DOAJ Directory of Open Access Journals customDbUrl: eissn: 1471-2407 dateEnd: 99991231 omitProxy: false ssIdentifier: ssj0017808 issn: 1471-2407 databaseCode: DOA dateStart: 20010101 isFulltext: true titleUrlDefault: https://www.doaj.org/ providerName: Directory of Open Access Journals – providerCode: PRVHPJ databaseName: ROAD: Directory of Open Access Scholarly Resources customDbUrl: eissn: 1471-2407 dateEnd: 99991231 omitProxy: false ssIdentifier: ssj0017808 issn: 1471-2407 databaseCode: M~E dateStart: 20010101 isFulltext: true titleUrlDefault: https://road.issn.org providerName: ISSN International Centre – providerCode: PRVPQU databaseName: Health & Medical Collection customDbUrl: eissn: 1471-2407 dateEnd: 99991231 omitProxy: false ssIdentifier: ssj0017808 issn: 1471-2407 databaseCode: 7X7 dateStart: 20090101 isFulltext: true titleUrlDefault: https://search.proquest.com/healthcomplete providerName: ProQuest – providerCode: PRVPQU databaseName: ProQuest Central customDbUrl: eissn: 1471-2407 dateEnd: 99991231 omitProxy: false ssIdentifier: ssj0017808 issn: 1471-2407 databaseCode: BENPR dateStart: 20090101 isFulltext: true titleUrlDefault: https://www.proquest.com/central providerName: ProQuest – providerCode: PRVPQU databaseName: Publicly Available Content Database customDbUrl: eissn: 1471-2407 dateEnd: 99991231 omitProxy: false ssIdentifier: ssj0017808 issn: 1471-2407 databaseCode: PIMPY dateStart: 20090101 isFulltext: true titleUrlDefault: http://search.proquest.com/publiccontent providerName: ProQuest – providerCode: PRVAVX databaseName: SpringerLink customDbUrl: eissn: 1471-2407 dateEnd: 99991231 omitProxy: false ssIdentifier: ssj0017808 issn: 1471-2407 databaseCode: RSV dateStart: 20011201 isFulltext: true titleUrlDefault: https://link.springer.com/search?facet-content-type=%22Journal%22 providerName: Springer Nature
link	http://cvtisr.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwnV1Lb9QwELZoixAX3o9AWQxC4kAt4sSxnWMLrdpDV6stoHKyHD_KSiVBm21_P2NvEkh5SHCJlHgsxZN5fJOxZxB6JVIhXF5ZkjKjCSvgUvG8Is4bbiqIoKm1sdmEmE7l6Wk56w6Ftf1u9z4lGS11VGvJ37ZgSWU4TZwRgAWMk3IDbYG7k0Ed5yefhtyBkKnsj8f8dt7IBcVK_b_a458c0tXNklcyptERHdz-vyXcQbc64Il315JyF11z9T1047hLrd9Hh6F1Z19MFjceL2p8uVgtG5yT9zg2zMEAcPE5WAdsgqwsSfjrj7-6lQaI2S5aHGvVPkAfD_Y_vDskXZsFYrjIVsRIXVlaOCFKnxtAILr0qfeMiSwtNACMjIaNsNSUeQrRR16UzBtnLUC3yvqsyB-izbqp3WOEvTVCC1dID16POqshntMilzZ3PINIL0G057wyXQ3y0ArjXMVYRHK1ZpECFqnIIlUm6M0w59u6AsdfqffCBx0oQ_Xs-KBZnqlOGRWtjAfoBMhYS-Yth-VzWhW-zCzVAHAT9DyIg1ofRR1sgNoVITNVMJom6GWkCBU06rBF50xftK06OpmPiF53RL6BVRrdnXgAXoWiWyPK7RElqLgZD_dyqToT0ypAVpynouSw5hfDcJgZts3VrrkINAUL7aSFTNCjtRgPnMkLxkrALwkSIwEfsW48Ui--xALkZRr7syRopxfzH6_150_z5N_In6KbWdQURjK6jTZBA9wzdN1crhbtcoI2xKmIVzlBW3v709l8Ev-nwN3s6Hj2eRKNwnda7VUw
linkProvider	Springer Nature
linkToHtml	http://cvtisr.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMw1V1Lb9QwELaqgoAL70egUINAHMBqnIcdHxAqlGpXfQhBK-3NOH6UlUpSNtsi_hS_kbGTbEkRvfXAJYf1RIrtmW9m1uP5EHrOY85tWhoSZ1qRLIdHydKSWKeZLiGDpsYEsgm-u1tMJuLjEvrV34XxZZU9JgagNrX2_5GvgSNhLOaCibdH34lnjfKnqz2FRqsWW_bnD0jZmjfjDdjfF0my-WHv_Yh0rAJEM57MiS5UaWhuORcu1eBwlXCxc1nGkzhX4E8T6us-qRZpDMF2movMaWsMRCqlcYlniQDIvwQ4zn0JGZ8sEjzKi7joL-YUbK0B7C_8_eeEQCCTMSIGzi9wBPztCf5whWfLNM-c1QYXuHnjf1u8m-h6F2zj9dY6bqElW91GV3a6coI7aOTpSvsGurh2eFrhk-l8VuOUbOBAEoQhqMeHgIhYe_uYEX_Sgb_ZuYKwupk2OPTnvYv2L2Qe99ByVVf2AcLOaK64zQsHnp5aoyCHVTwtTGpZAtlthGi_51J3fdc9_cehDPlXwWSrJxL0RAY9kSJCrxbvHLVdR86VfudVaSHpO4aHH-rZgewASNJSOwgXIRtQReYMg-kzWuZOJIYqCOojtOoVUbbXbxe4J9e5P43LMxpH6FmQ8F1DKl-WdKCOm0aOP38aCL3shFwNs9Squ-UBa-UbjQ0kVwaSAGt6ONyrsuxgtZGnehyhp4th_6YvFaxsfexl8sxTaPMiQvdbA1qsTJpnmYCYLUJ8YFqDpRuOVNOvoem6iAMnTYRe90Z4-ln_3pqH589iFV0d7e1sy-3x7tYjdC0JUJGRhK6gZdB--xhd1ifzaTN7EoAGoy8XbZy_AS6FtBY
linkToPdf	http://cvtisr.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwpV1Zb9QwELagoIoX7iNQqEFIPFCrORwfj4WyagWsKgqob5bjo6xUkmqz7e9n7Bw05ZAQL_sQj6X1eGb8jeZC6CVPOXdFZUlKjSa0hJ-KFRVx3jBTgQedWRuHTfD5XBwdyYMLVfwx230ISXY1DaFLU73aPrW-U3HBtluwqiJUFucEIAJlRF5F12gYGhT89cOvYxyBi1QMpTK_3Td5jmLX_l9t84XH6XLi5KXoaXyUZrf-_zi30c0ekOKdToLuoCuuvovWP_Yh93toL4z0HJrM4sbjRY3PF6tlgwuyi-MgHQzAF5-A1cAmyNCShGgA_u5WGqBnu2hx7GF7H32Zvfv8do_04xeIYTxfESN0ZbPScS59YQCZaOlT7ynleVpqAB55FhJkMyOLFLySopTUG2ctQLrK-rwsHqC1uqndI4S9NVxzVwoPr2HmrAY_T_NC2MKxHDzABGXDLSjT9yYPIzJOVPRRBFMdixSwSEUWKZmg1-Oe064zx1-p34TLHSlDV-34oVkeq15JVVYZD5AKELMW1FsGx2dZVXqZ20wD8E3QZhAN1ZWojrZB7fAQsSpBABP0IlKEzhp1SN051mdtq_YPP02IXvVEvoFTGt1XQgCvQjOuCeXGhBJU30yXBxlVvelpFSAuxlIuGZz5-bgcdoZ0uto1Z4GmpGHMNBcJetiJ9MiZoqRUAq5JEJ8I-4R105V68S02JpdpnNuSoK1B5H_-rT9fzeN_I99E6we7M_Vhf_7-CbqRR6WhJM820Boog3uKrpvz1aJdPouW4AeiB1ro
openUrl	ctx_ver=Z39.88-2004&ctx_enc=info%3Aofi%2Fenc%3AUTF-8&rfr_id=info%3Asid%2Fsummon.serialssolutions.com&rft_val_fmt=info%3Aofi%2Ffmt%3Akev%3Amtx%3Ajournal&rft.genre=article&rft.atitle=Construction+of+in+vitro+3-D+model+for+lung+cancer-cell+metastasis+study&rft.jtitle=BMC+cancer&rft.au=Jiang%2C+Rongrong&rft.au=Huang%2C+Jiechun&rft.au=Sun%2C+Xiaotian&rft.au=Chu%2C+Xianglin&rft.date=2022-04-21&rft.pub=BioMed+Central&rft.eissn=1471-2407&rft.volume=22&rft.issue=1&rft_id=info:doi/10.1186%2Fs12885-022-09546-9&rft.externalDocID=10_1186_s12885_022_09546_9
thumbnail_l	http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/lc.gif&issn=1471-2407&client=summon
thumbnail_m	http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/mc.gif&issn=1471-2407&client=summon
thumbnail_s	http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/sc.gif&issn=1471-2407&client=summon