Challenges of the Human Proteome Project: 10-Year Experience of the Russian Consortium

被引:7
作者
Archakov, Alexander I. [1 ]
Aseev, Alexander L. [2 ]
Bykov, Victor A. [3 ]
Grigoriev, Anatoly I. [4 ]
Govorun, Vadim M. [5 ]
Ilgisonis, Ekaterina V. [1 ]
Ivanov, Yuri D. [1 ]
Ivanov, Vadim T. [6 ]
Kiseleva, Olga I. [1 ]
Kopylov, Arthur T. [1 ]
Lisitsa, Andrey V. [1 ]
Mazurenko, Sergey N. [7 ]
Makarov, Alexander A. [8 ]
Naryzhny, Stanislav N. [1 ]
Pleshakova, Tatiana O. [1 ]
Ponomarenko, Elena A. [1 ]
Poverennaya, Ekaterina V. [1 ]
Pyatnitskii, Mikhail A. [1 ]
Sagdeev, Renad Z. [9 ]
Skryabin, Konstantin G. [10 ]
Zgoda, Victor G. [1 ]
机构
[1] Inst Biomed Chem, Moscow 119435, Russia
[2] Inst Semicond Phys, Novosibirsk 630090, Russia
[3] NT MDT, Moscow 124460, Russia
[4] Inst Med & Biol Problems, Moscow 123007, Russia
[5] Fed Res & Clin Ctr Phys Chem Med, Moscow 119435, Russia
[6] Shemyakin Ovchinnikov Inst Bioorgan Chem, Moscow 117997, Russia
[7] Joint Inst Nucl Res, Dubna 141980, Moscow Region, Russia
[8] Engelhardt Inst Mol Biol, Moscow 119991, Russia
[9] Int Tomog Ctr, Novosibirsk 630090, Russia
[10] Fed Res Ctr Fundamentals Biotechnol, Moscow 119071, Russia
关键词
human proteome; mass-spectrometry; Chromosome-Centric Human Proteome Project (C-HPP); sensitivity; fractionation; missing proteins; atomic force microscopy; proteoforms; low-abundant proteins; ATOMIC-FORCE MICROSCOPY; MASS-SPECTROMETRY; MESSENGER-RNA; LIVER-TISSUE; DEPLETED PLASMA; TRANSCRIPTOME; SPECIFICITY; GENERATION; NANOWIRE; NUMBER;
D O I
10.1021/acs.jproteome.9b00358
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
This manuscript collects all the efforts of the Russian Consortium, bottlenecks revealed in the course of the C-HPP realization, and ways of their overcoming. One of the main bottlenecks in the C-HPP is the insufficient sensitivity of proteomic technologies, hampering the detection of low- and ultralow-copy number proteins forming the "dark part" of the human proteome. In the frame of MP-Challenge, to increase proteome coverage we suggest an experimental workflow based on a combination of shotgun technology and selected reaction monitoring with two-dimensional alkaline fractionation. Further, to detect proteins that cannot be identified by such technologies, nanotechnologies such as combined atomic force microscopy with molecular fishing and/or nanowire detection may be useful. These technologies provide a powerful tool for single molecule analysis, by analogy with nanopore sequencing during genome analysis. To systematically analyze the functional features of some proteins (CP50 Challenge), we created a mathematical model that predicts the number of proteins differing in amino acid sequence: proteoforms. According to our data, we should expect about 100 000 different proteoforms in the liver tissue and a little more in the HepG2 cell line. The variety of proteins forming the whole human proteome significantly exceeds these results due to post-translational modifications (PTMs). As PTMs determine the functional specificity of the protein, we propose using a combination of gene-centric transcriptome-proteomic analysis with preliminary fractionation by two-dimensional electrophoresis to identify chemically modified proteoforms. Despite the complexity of the proposed solutions, such integrative approaches could be fruitful for MP50 and CP50 Challenges in the framework of the C-HPP.
引用
收藏
页码:4206 / 4214
页数:9
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