APA
Gonzalez Barderas, Maria & Gallego-Delgado, Julio & Mas, Sebastián & Duran, Mari Carmen & Lázaro, Alberto & Hernandez Merida, Sergio & Egido, Jesús & Vivanco, Fernando, Fernando Vivanco .Isolation of circulating human monocytes with high purity for proteomic analysis.
ISO 690
Gonzalez Barderas, Maria & Gallego-Delgado, Julio & Mas, Sebastián & Duran, Mari Carmen & Lázaro, Alberto & Hernandez Merida, Sergio & Egido, Jesús & Vivanco, Fernando. Isolation of circulating human monocytes with high purity for proteomic analysis.
https://hdl.handle.net/20.500.12080/39714
Abstract:
We describe a simple method for isolation of human blood monocytes with the high
purity (95¿98%) required for proteomic analysis, which avoids contamination by other
blood cells (platelets and lymphocytes) and the most abundant plasma proteins (albu min and immunoglobulins). Blood monocytes were purified by gradient centrifugation
followed by positive selection with specific monoclonal antibodies coupled to para magnetic beads. The elution conditions of the positive selection step were modified
to avoid contamination with albumin. This method is compatible with flow cytometry
which was used to assess the purity of the cell population. From 28 mL of blood, 107
monocytes with . 96% purity are routinely obtained. From the isolated monocytes
200¿250 mg of protein could be recovered. The whole method can be performed in
three hours. Similar results were obtained using a negative selection step but with
lower purity (92%), increased cost and longer time. After solubilization of monocytes,
the proteins were analyzed by two-dimensional gel electrophoresis (2-DE) in the 3¿10,
4¿7, 6¿9 and 6¿11 pH range. DNA was the main contaminant that interfered with the 2-
DE and it was removed by treatment with DNAse. Image analysis of gels allowed the
reproducible detection and quantification of 1500 spots in the 4¿7 pH range and more
than 2000 spots in total by combining (overlapping) 2-D gels in the 4¿7, 6¿9 and
6¿11 pH range. This method is useful for clinical studies of monocytes from a large
number of patients due to its rapidity and reproducibility, which permits comparative
analysis of normal versus pathological samples and which allows follow up of the
expressed proteins of monocytes from each patient.
Keywords: Human monocytes / Isolation method / Proteomic analysis / Two-dimensional gel
electrophoresis