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Featured researches published by -Lin Chen.


Biosensors and Bioelectronics | 2008

A planar interdigitated ring electrode array via dielectrophoresis for uniform patterning of cells

Lo-Chang Hsiung; Chun-Hui Yang; Chi-Li Chiu; Chen-Lin Chen; Yueh Wang; Hsinyu Lee; Ji-Yen Cheng; Ming-Chih Ho; Andrew M. Wo

Uniform patterning of cells is highly desirable for most cellular studies involving cell-cell interactions but is often difficult in an in vitro environment. This paper presents the development of a collagen-coated planar interdigitated ring electrode (PIRE) array utilizing positive dielectrophoresis to pattern cells uniformly. Key features of the PIRE design include: (1) maximizing length along the edges where the localized maximum in the electric field exists; (2) making the inner gap slightly smaller than the outer gap in causing the electric field strength near the center of a PIRE being generally stronger than that near the outer edge of the same PIRE. Results of human hepatocellular carcinoma cells, HepG2, adhered on a 6x6 PIRE array show that cells patterned within minutes with good uniformity (48+/-6 cells per PIRE). Cell viability test revealed healthy patterned cells after 24h that were still confined to the collagen-coated PIREs. Furthermore, quantification of fluorescence intensity of living cells shows an acceptable reproducibility of cell viability among PIREs (mean normalized intensity per PIRE was 1+/-0.138). The results suggest that the PIRE array would benefit applications that desire uniform cellular patterning, and improve both response and reproducibility of cell-based biosensors.


Clinical Chemistry | 2011

Detection of Circulating Endothelial Cells via a Microfluidic Disk

Ken-Chao Chen; Tai-Ping Lee; Yu-Cheng Pan; Chi-Ling Chiang; Chen-Lin Chen; Yao-Hsu Yang; Bor-Luen Chiang; Hsinyu Lee; Andrew M. Wo

BACKGROUND Circulating endothelial cells (CECs) in the blood are rare but have been shown to be associated with various diseases. With the ratio of CECs to peripheral blood mononuclear cells (PBMCs) less than 1 part per thousand, their separation from PBMCs and detection are challenging. We present a means of detecting CECs from PBMCs via an economical microfluidic disk with a model cell system [human umbilical vein endothelial cells (HUVECs) in PBMCs], along with demonstration of its efficacy clinically. METHODS To enrich these rare cells, we used immunomagnetic beads and a tailor-made magnet on the disk. CEC-simulating HUVECs, as target cells, were stained with primary anti-CD146-phycoerythrin antibody and bound with secondary antibody on antiphycoerythrin magnetic beads. PBMCs served as nontarget cells and were labeled with anti-CD45-FITC antibody. RESULTS When hundreds of HUVECs were mixed in 10(6) PBMCs, 95% of spiked HUVECs were detected. This yield also held for 60 HUVEC in <10(4) PBMCs. We compared data from flow cytometry with that from the disk: CEC counts in 50 μL blood from patients with systemic lupus erythematosus were 61.1 (21.5), significantly higher (P < 0.01) than those of healthy donors, 31.2 (13.3). CONCLUSIONS The count of CECs is a suitable marker for symptoms of systemic lupus erythematosus. The microfluidic disk system should be a viable platform for detection of CECs.


Analytical Biochemistry | 2012

Enumeration and viability of rare cells in a microfluidic disk via positive selection approach

Ken-Chao Chen; Yu-Cheng Pan; Chen-Lin Chen; Ching-Hung Lin; Chiun-Sheng Huang; Andrew M. Wo

Recent studies have shown that specific rare cells in the blood can serve as an indicator of cancer prognosis, among other purposes. This article demonstrates the concept of separating and detecting rare cells from peripheral blood mononuclear cells via an economical microfluidic disk with a model system. MCF7, labeled with magnetic beads, was used to simulate circulating tumor cells as a target. Jurkat clone E6-1 was used to simulate leukocytes or other cells abundant in human blood. A tailored multistage magnet maximized the magnetic field to ensure optimal trapping efficiency. Results indicate that the yield of detected MCF7 was consistent at approximately 80% when fewer than hundreds of MCF7 cells were mixed in greater than 1 million Jurkat cells. The 80% yield also held for 10 MCF7 in 100 million Jurkat (rarity of 10(7)). Compared with the results from autoMACS, the performance was at least 20% higher and was more independent of the number of Jurkat. The viability of the enriched cells was approximately 90 ± 20%, showing that this method caused little damage to trapped cells. The microfluidic disk should be applicable for separation and detection of various rare cells, such as circulating tumor cells and circulating endothelial cells in human blood.


nano/micro engineered and molecular systems | 2011

Modeling of circulating tumor cells via cell lines and mononuclear cells in a microfluidic disk

Chen-Lin Chen; Yu-Cheng Pan; Ken-Chao Chen; Andrew M. Wo

Cyto-analysis of rare cells often requires separation and detection with either procedure possesses substantial challenge. This paper presents a disk-based microfluidic platform for both procedures via immunomagnetic negative selection process. Proof-of-concept was conducted using wide range of MCF7 as target rare cells and spiked into Jurkat as non-target cells. Then, mononuclear cells (MNC) from healthy blood donors were mixed with MCF7s, modeling rare cells, and tested in the disk. Results show the average yield of detected MCF7 is near-constant 60±10% over a wide range of rarity from 10−3 to 10−6 and this yield also holds for MCF7/MNC complex mixture. Comparison with autoMACS and BD IMagnet separators revealed the average yield from the disk (60%) is superior to that of autoMACS (37.3%) and BD IMagnet (48.3%).


Lab on a Chip | 2011

Separation and detection of rare cells in a microfluidic disk via negative selection

Chen-Lin Chen; Ken-Chao Chen; Yu-Cheng Pan; Tai-Ping Lee; Lo-Chang Hsiung; Cheng-Ming Lin; Chang-Yu Chen; Ching-Hung Lin; Bor-Luen Chiang; Andrew M. Wo


Archive | 2009

Compact disk based platform for separating and detecting immunomagnetic bead labeled cells

Andrew M. Wo; Chen-Lin Chen; Ken-Chao Chen; Yu-Cheng Pan


Journal of Food Science | 2006

Process Characteristics of Hydrolysis of Chitosan in a Continuous Enzymatic Membrane Reactor

Chia-Hung Kuo; Chen-Lin Chen; Been‐Huang Chiang


Journal of Food Science | 2002

Characterization of Lactoferrin (LF) from Colostral Whey Using Anti-LF Antibody Immunoaffinity Chromatography

Y.-Y. Tu; Chen-Lin Chen; Jung-Yu Chang; Hsu-Hsien Chang


Analyst | 2014

A spatiotemporally defined in vitro microenvironment for controllable signal delivery and drug screening

Ching-Te Kuo; Hao-Kai Liu; Guan-Syuan Huang; Chi-Hao Chang; Chen-Lin Chen; Ken-Chao Chen; Ruby Yun-Ju Huang; Ching-Hung Lin; Hsinyu Lee; Chiun-Sheng Huang; Andrew M. Wo


Archive | 2009

Compact disk based system for separating immunomagnetic bead labeled particulates and method thereof

Andrew M. Wo; Chen-Lin Chen; Ken-Chao Chen; Yu-Cheng Pan

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Andrew M. Wo

National Taiwan University

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Ken-Chao Chen

National Taiwan University

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Yu-Cheng Pan

National Taiwan University

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Ching-Hung Lin

National Taiwan University

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Cheng-Wei Yang

National Taiwan University

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Chiun-Sheng Huang

National Taiwan University

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Hsinyu Lee

National Taiwan University

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Lo-Chang Hsiung

National Taiwan University

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Bor-Luen Chiang

National Taiwan University

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Chang-Yu Chen

National Taiwan University

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