Study of differential proteins in lung adenocarcinoma using laser capture microdissection combined with liquid chip-mass spectrometry technology

Li Na Bu; Shuan Ying Yang; Feng Tao Li; Wen Li Shang; Wei Zhang; Shu Fen Huo; Yan Dong Nan; Ying Xuan Tian; Jie Du; Xiu Li Lin; Yan Feng Liu; Yu Rong Lin; Biao Xue Rong

doi:10.3760/cma.j.issn.0366-6999.2010.22.026

Study of differential proteins in lung adenocarcinoma using laser capture microdissection combined with liquid chip-mass spectrometry technology

Li Na Bu
, Shuan Ying Yang
, Feng Tao Li
, Wen Li Shang
, Wei Zhang
, Shu Fen Huo
, Yan Dong Nan
, Ying Xuan Tian
, Jie Du
, Xiu Li Lin
, Yan Feng Liu
, Yu Rong Lin
, Biao Xue Rong

Health Science Center

Xi'an Jiaotong University
Xi'an Central Hospital

Research output: Contribution to journal › Article › peer-review

3 Scopus citations

Abstract

Background In recent years the proportion of lung adenocarcinoma (adCA) which occurs in lung cancer patients has increased. Using laser capture microdissection (LCM) combined with liquid chip-mass spectrometry technology, we aimed to screen lung cancer biomarkers by studying the proteins in the tissues of adCA. Methods We used LCM and magnetic bead based weak cation exchange (MB-WCX) to separate and purify the homogeneous adCA cells and normal cells from six cases of fresh adCA and matched normal lung tissues. The proteins were analyzed and identified by matrix assisted laser desorption/ionization time-of-fight mass spectrometry (MALDI-OF-MS). We screened for the best pattern using a radial basic function neural network algorithm. Results About 2.895×10⁶ and 1.584×10⁶ cells were satisfactorily obtained by LCM from six cases of fresh lung adCA and matched normal lung tissues, respectively. The homogeneities of cell population were estimated to be over 95% as determined by microscopic visualization. Comparing the differentially expressed proteins between the lung adCA and the matched normal lung group, 221 and 239 protein peaks, respectively, were found in the mass-to-charge ration (M/Z) between 800 Da and 10 000 Da. According to t test, the expression of two protein peaks at 7521.5 M/Z and 5079.3 M/Z had the largest difference between tissues. They were more weakly expressed in the lung adCA compared to the matched normal group. The two protein peaks could accurately separate the lung adCA from the matched normal lung group by the sample distribution chart. A discriminatory pattern which can separate the lung adCA from the matched normal lung tissue consisting of three proteins at 3358.1 M/Z, 5079.3 M/Z and 7521.5 M/Z was established by a radial basic function neural network algorithm with a sensitivity of 100% and a specificity of 100%. Conclusions Differential proteins in lung adCA were screened using LCM combined with liquid chip-mass spectrometry technology, and a biomarker model was established. It is possible that this technology is going to become a powerful tool in screening and early diagnosis of lung adCA.

Original language	English
Pages (from-to)	3309-3313
Number of pages	5
Journal	Chinese Medical Journal
Volume	123
Issue number	22
DOIs	https://doi.org/10.3760/cma.j.issn.0366-6999.2010.22.026
State	Published - 20 Nov 2010

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

SDG 3 Good Health and Well-being

Keywords

Laser capture microdissection
Lung adenocarcinoma
Magnetic beads
Mass spectrometry

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10.3760/cma.j.issn.0366-6999.2010.22.026

Cite this

Bu, L. N., Yang, S. Y., Li, F. T., Shang, W. L., Zhang, W., Huo, S. F., Nan, Y. D., Tian, Y. X., Du, J., Lin, X. L., Liu, Y. F., Lin, Y. R., & Rong, B. X. (2010). Study of differential proteins in lung adenocarcinoma using laser capture microdissection combined with liquid chip-mass spectrometry technology. Chinese Medical Journal, 123(22), 3309-3313. https://doi.org/10.3760/cma.j.issn.0366-6999.2010.22.026

@article{4b93e7f41e1b4a528e811f4f5536c874,

title = "Study of differential proteins in lung adenocarcinoma using laser capture microdissection combined with liquid chip-mass spectrometry technology",

abstract = "Background In recent years the proportion of lung adenocarcinoma (adCA) which occurs in lung cancer patients has increased. Using laser capture microdissection (LCM) combined with liquid chip-mass spectrometry technology, we aimed to screen lung cancer biomarkers by studying the proteins in the tissues of adCA. Methods We used LCM and magnetic bead based weak cation exchange (MB-WCX) to separate and purify the homogeneous adCA cells and normal cells from six cases of fresh adCA and matched normal lung tissues. The proteins were analyzed and identified by matrix assisted laser desorption/ionization time-of-fight mass spectrometry (MALDI-OF-MS). We screened for the best pattern using a radial basic function neural network algorithm. Results About 2.895×106 and 1.584×106 cells were satisfactorily obtained by LCM from six cases of fresh lung adCA and matched normal lung tissues, respectively. The homogeneities of cell population were estimated to be over 95\% as determined by microscopic visualization. Comparing the differentially expressed proteins between the lung adCA and the matched normal lung group, 221 and 239 protein peaks, respectively, were found in the mass-to-charge ration (M/Z) between 800 Da and 10 000 Da. According to t test, the expression of two protein peaks at 7521.5 M/Z and 5079.3 M/Z had the largest difference between tissues. They were more weakly expressed in the lung adCA compared to the matched normal group. The two protein peaks could accurately separate the lung adCA from the matched normal lung group by the sample distribution chart. A discriminatory pattern which can separate the lung adCA from the matched normal lung tissue consisting of three proteins at 3358.1 M/Z, 5079.3 M/Z and 7521.5 M/Z was established by a radial basic function neural network algorithm with a sensitivity of 100\% and a specificity of 100\%. Conclusions Differential proteins in lung adCA were screened using LCM combined with liquid chip-mass spectrometry technology, and a biomarker model was established. It is possible that this technology is going to become a powerful tool in screening and early diagnosis of lung adCA.",

keywords = "Laser capture microdissection, Lung adenocarcinoma, Magnetic beads, Mass spectrometry",

author = "Bu, \{Li Na\} and Yang, \{Shuan Ying\} and Li, \{Feng Tao\} and Shang, \{Wen Li\} and Wei Zhang and Huo, \{Shu Fen\} and Nan, \{Yan Dong\} and Tian, \{Ying Xuan\} and Jie Du and Lin, \{Xiu Li\} and Liu, \{Yan Feng\} and Lin, \{Yu Rong\} and Rong, \{Biao Xue\}",

year = "2010",

month = nov,

day = "20",

doi = "10.3760/cma.j.issn.0366-6999.2010.22.026",

language = "英语",

volume = "123",

pages = "3309--3313",

journal = "Chinese Medical Journal",

issn = "0366-6999",

publisher = "Lippincott Williams and Wilkins",

number = "22",

}

Bu, LN, Yang, SY, Li, FT, Shang, WL, Zhang, W, Huo, SF, Nan, YD, Tian, YX, Du, J, Lin, XL, Liu, YF, Lin, YR & Rong, BX 2010, 'Study of differential proteins in lung adenocarcinoma using laser capture microdissection combined with liquid chip-mass spectrometry technology', Chinese Medical Journal, vol. 123, no. 22, pp. 3309-3313. https://doi.org/10.3760/cma.j.issn.0366-6999.2010.22.026

TY - JOUR

T1 - Study of differential proteins in lung adenocarcinoma using laser capture microdissection combined with liquid chip-mass spectrometry technology

AU - Bu, Li Na

AU - Yang, Shuan Ying

AU - Li, Feng Tao

AU - Shang, Wen Li

AU - Zhang, Wei

AU - Huo, Shu Fen

AU - Nan, Yan Dong

AU - Tian, Ying Xuan

AU - Du, Jie

AU - Lin, Xiu Li

AU - Liu, Yan Feng

AU - Lin, Yu Rong

AU - Rong, Biao Xue

PY - 2010/11/20

Y1 - 2010/11/20

N2 - Background In recent years the proportion of lung adenocarcinoma (adCA) which occurs in lung cancer patients has increased. Using laser capture microdissection (LCM) combined with liquid chip-mass spectrometry technology, we aimed to screen lung cancer biomarkers by studying the proteins in the tissues of adCA. Methods We used LCM and magnetic bead based weak cation exchange (MB-WCX) to separate and purify the homogeneous adCA cells and normal cells from six cases of fresh adCA and matched normal lung tissues. The proteins were analyzed and identified by matrix assisted laser desorption/ionization time-of-fight mass spectrometry (MALDI-OF-MS). We screened for the best pattern using a radial basic function neural network algorithm. Results About 2.895×106 and 1.584×106 cells were satisfactorily obtained by LCM from six cases of fresh lung adCA and matched normal lung tissues, respectively. The homogeneities of cell population were estimated to be over 95% as determined by microscopic visualization. Comparing the differentially expressed proteins between the lung adCA and the matched normal lung group, 221 and 239 protein peaks, respectively, were found in the mass-to-charge ration (M/Z) between 800 Da and 10 000 Da. According to t test, the expression of two protein peaks at 7521.5 M/Z and 5079.3 M/Z had the largest difference between tissues. They were more weakly expressed in the lung adCA compared to the matched normal group. The two protein peaks could accurately separate the lung adCA from the matched normal lung group by the sample distribution chart. A discriminatory pattern which can separate the lung adCA from the matched normal lung tissue consisting of three proteins at 3358.1 M/Z, 5079.3 M/Z and 7521.5 M/Z was established by a radial basic function neural network algorithm with a sensitivity of 100% and a specificity of 100%. Conclusions Differential proteins in lung adCA were screened using LCM combined with liquid chip-mass spectrometry technology, and a biomarker model was established. It is possible that this technology is going to become a powerful tool in screening and early diagnosis of lung adCA.

AB - Background In recent years the proportion of lung adenocarcinoma (adCA) which occurs in lung cancer patients has increased. Using laser capture microdissection (LCM) combined with liquid chip-mass spectrometry technology, we aimed to screen lung cancer biomarkers by studying the proteins in the tissues of adCA. Methods We used LCM and magnetic bead based weak cation exchange (MB-WCX) to separate and purify the homogeneous adCA cells and normal cells from six cases of fresh adCA and matched normal lung tissues. The proteins were analyzed and identified by matrix assisted laser desorption/ionization time-of-fight mass spectrometry (MALDI-OF-MS). We screened for the best pattern using a radial basic function neural network algorithm. Results About 2.895×106 and 1.584×106 cells were satisfactorily obtained by LCM from six cases of fresh lung adCA and matched normal lung tissues, respectively. The homogeneities of cell population were estimated to be over 95% as determined by microscopic visualization. Comparing the differentially expressed proteins between the lung adCA and the matched normal lung group, 221 and 239 protein peaks, respectively, were found in the mass-to-charge ration (M/Z) between 800 Da and 10 000 Da. According to t test, the expression of two protein peaks at 7521.5 M/Z and 5079.3 M/Z had the largest difference between tissues. They were more weakly expressed in the lung adCA compared to the matched normal group. The two protein peaks could accurately separate the lung adCA from the matched normal lung group by the sample distribution chart. A discriminatory pattern which can separate the lung adCA from the matched normal lung tissue consisting of three proteins at 3358.1 M/Z, 5079.3 M/Z and 7521.5 M/Z was established by a radial basic function neural network algorithm with a sensitivity of 100% and a specificity of 100%. Conclusions Differential proteins in lung adCA were screened using LCM combined with liquid chip-mass spectrometry technology, and a biomarker model was established. It is possible that this technology is going to become a powerful tool in screening and early diagnosis of lung adCA.

KW - Laser capture microdissection

KW - Lung adenocarcinoma

KW - Magnetic beads

KW - Mass spectrometry

UR - https://www.scopus.com/pages/publications/79251523492

U2 - 10.3760/cma.j.issn.0366-6999.2010.22.026

DO - 10.3760/cma.j.issn.0366-6999.2010.22.026

M3 - 文章

C2 - 21163136

AN - SCOPUS:79251523492

SN - 0366-6999

VL - 123

SP - 3309

EP - 3313

JO - Chinese Medical Journal

JF - Chinese Medical Journal

IS - 22

ER -

Study of differential proteins in lung adenocarcinoma using laser capture microdissection combined with liquid chip-mass spectrometry technology

Abstract

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Keywords

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