This study analyzed single-nuclei transcriptomes of thirty-three individuals with Alzheimer’s disease (AD), revealing sex-specific DEGs in glial cells. Functional enrichment analysis highlighted synaptic, neural, and hormone-related pathways. Key genes, namely NLGN4Y and its regulators, were identified, and potential therapeutic candidates for gender-specific AD were proposed.
Many sex-specific biomarkers have been recently revealed in Alzheimer's disease (AD); however, cerebral glial cells were rarely reported. This study analyzed 220,095 single-nuclei transcriptomes from the frontal cortex of thirty-three AD individuals in the GEO database. Sex-specific Differentially Expressed Genes (DEGs) were identified in glial cells, including 243 in astrocytes, 1,154 in microglia, and 572 in oligodendrocytes. Gene Ontology (GO) functional annotation analyses and Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway enrichment analyses revealed functional concentration in synaptic, neural, and hormone-related pathways. Protein-protein interaction network (PPI) identified MT3, CALM2, DLG2, KCND2, PAKACB, CAMK2D, and NLGN4Y in astrocytes, TREM2, FOS, APOE, APP, and NLGN4Y in microglia, and GRIN2A, ITPR2, GNAS, and NLGN4Y in oligodendrocytes as key genes. NLGN4Y was the only gene shared by the three glia and was identified as the biomarker for the gender specificity of AD. Gene-transcription factor (TF)-miRNA coregulatory network identified key regulators for NLGN4Y and its target TCMs. Ecklonia kurome Okam (Kunbu) and Herba Ephedrae (Mahuang) were identified, and the effects of the active ingredients on AD were displayed. Finally, enrichment analysis of Kunbu and Mahuang suggested that they might act as therapeutic candidates for gender specificity of AD.
Alzheimer's disease (AD) is a global disease with high incidence, and it accounts for 60%-80% of dementia1. Despite its high incidence, the mechanistic pathogenesis of AD is not clearly delineated, and there have been no effective therapeutics until now2. The main pathologies in AD were identified as neuronal atrophy and the accumulation of pathological debris, mainly microtubule-associated protein Tau, and β-amyloid (Aβ)3,4. The pathogenesis of AD is associated with abnormal autophagy, oxidative stress, mitochondrial dysfunction, inflammation, and energy metabolism disorder5. Prevalence surveys proved that two-thirds of AD patients were women6. Sex-specific differences in AD exist in the etiology, clinical manifestations, prevention, and treatment. Thus, revealing the biological mechanism that causes sex-specific differences in AD and targeting traditional Chinese medicine (TCM) can potentially provide a more comprehensive theoretical framework to understand the pathogenesis of AD, and to further guide accurate treatment strategy.
Neuroglial cells, especially microglia, astrocytes, and oligodendrocytes, potentially contribute to the pathogenesis of AD. In AD, microglia are activated and genetically altered, which contribute to inflammatory response, phagocytosis, and Aβ clearance7,8; astrocyte is genetically altered, which affects synaptic activity, ion homeostasis, and energy and lipid metabolism9; oligodendrocyte is genetically altered with sex specificity, which contributes to neuronal loss, neurofibrillary tangles, and white matter lesions10,11.
In this study, we employed single-nuclei RNA sequencing (snRNA-seq) as a superior technique. Compared to single-cell RNA sequencing (scRNA-seq), snRNA-seq offers advantages in terms of sample richness, cell type integrity, and data reliability12,13. SnRNA-seq has been extensively utilized in studies focusing on AD and exploring the role of glial cells14,15,16. Its wide adoption in these research areas highlights its effectiveness in providing valuable insights into the transcriptional characteristics of glial cells in AD. By leveraging the advantages of snRNA-seq, researchers have been able to uncover crucial information regarding the involvement of glial cells in AD pathology and identify potential therapeutic targets. In order to explore sex-specific neuroglial transcriptional characteristics in AD and potential TCMs for sex specificity of AD, this study analyzed snRNA-seq data from the frontal cortex of AD patients from the NCBI GEO public database. Sex-specific differentially expressed genes (DEGs), Gene Ontology (GO), Kyoto Encyclopedia of Genes and Genomes (KEGG), Protein-protein interaction (PPI) network, and gene-TF-miRNA network are further analyzed to reveal key biomarkers and potential pathogenesis. Finally, potential TCMs were suggested, and their active ingredients were displayed with tables by searching the Coremine Medical, TCMIP, and TCMSP databases.
Steps 2 to 9 of the analysis were implemented using R software (see Supplementary Figure 1 and Supplementary File 1), while the remaining steps were executed on the online platforms. The details of the databases used in this protocol (along with the weblinks) are provided in the Table of Materials.
1. Data acquisition
2. Sample merging
3. Quality control (QC)
4. Batch effect checking
5. Data integration
6. Cell type annotation
7. Glial cell data extraction
8. Glial sex-specific differentially expressed genes (DEGs) capturing
9. Functional enrichment analyses of sex-specific DEGs
10. Frequency statistics of glial DEGs in go and kegg pathways, venn diagrams of each glial sex-specific DEGs, and PPI network construction
11. Multifactor regulatory network construction
12. Gene and target TCM analysis
13. Research summary of TCM ingredients in targeting key gene
14. Confirming of targeting TCMs' treatment function in the sex specificity of AD
SnRNA-seq analysis of frontal glial transcriptome profiles and the annotation of cell types
In total, 220,095 nuclei and 32,077 genes in the frontal cortex of 17 male AD and 17 female AD were obtained (Figure 1A). UMAP plot visualized the total single-nuclei frontal transcriptomes displaying distinct types of nuclei after dimension reduction analysis (Figure 1B). Total numbers of annotated nuclei captured by gender were shown, which made the sum of included 58,902 astrocytes, 14,265 microglia, 77,466 oligodendrocytes, 3,520 endothelial, 25,252 excitatory neurons, 31,268 inhibitory neurons and 9,422 oligodendrocyte progenitor cells (Figure 1C). Average expressions of the known cell type markers for each glia were projected on the UMAP plots to identify the cell populations (Figure 1D).
The sex-specific DEGs in astrocytes
58,902 astrocytic nuclei were analyzed (Figure 2A), with 27,504 from male AD (46.69%) and 31,398 from female AD (53.31%). Sex-specific DEGs revealed upregulation of 138 genes, including DST, CACNA2D3, and AC016831.7, downregulation of 105 genes, including CNTN5, RORA, RASSF8, and CADM2, and unchanged 4995 genes (Figure 2B). Further, GO and KEGG analyses identified that those DEGs primarily concentrated in the pathways of neurons, synapses, and hormones, with neuronal pathways including regulation of neuron project development, neuron spine, etc., synaptic pathways including synaptic organization and glutamatergic/cholinergic synapse, and hormone pathways including thyroid hormone synthesis and insulin secretion (Figure 2C,D). Thirty genes with top frequency were obtained (Figure 2E), with PLCB1 ranking the first. PPI networks were constructed to explore the relationship between these genes (Figure 2F) and identified DLG2, CAMK2D, CALM2, and PRKACB as core genes. UMAP plots displayed differences of selected DEGs: KCND2, CAMK2D, MT3, LINC00278, and XIST were higher in female AD and lower in male AD, while NLGN4Y, DLG2, PRKACB, CALM2, UTY, and TTTY14 were opposite (Figure 2G). MT3, CALM2, DLG2, KCND2, PRKACB, CAMK2D, and NLGN4Y were finally determined as sex-specific DEGs of astrocytes as shown in Table 1.
The sex-specific DEGs in microglia
14,265 microglial nuclei (Figure 3A) were analyzed, with 5,327 (37.34%) from male AD and 8,938 (62.66%) from female AD. Sex-specific DEGs revealed upregulation of 224 genes, including KCNIP4 and LRRTM4, and downregulation of 930 genes, including APOE, MT-CO3, and FTL, and unchanged 13,111 genes (Figure 3B). Further, GO and KEGG analyses identified that those DEGs mainly concentrated in the pathways of neurons, phagosome, hormones, and others, with neuronal pathways including neuron-to-neuron synapse, phagocytic pathways including phagosome and regulation of phagocytosis, hormone pathways including estrogen signaling pathway, oxytocin signaling pathway, etc., and others including regulation of inflammatory response, learning or memory, amyloid-beta clearance, etc. (Figure 3C,D). Thirty genes with top frequency were obtained, with TLR2 and TREM2 tied for second place (Figure 3E). PPI networks were constructed to explore the relationship between these genes (Figure 3F) and identified ACTB, APP, and FYN as core genes. UMAP plots displayed differences of selected DEGs: APP, FOS, XIST, and CTSD were higher in female AD and lower in male AD, while NLGN4Y, TREM2, LINC0028, APOE, UTY and TTTY14 were opposite (Figure 3G). TREM2, FOS, APOE, APP, and NLGN4Y were finally determined as sex-specific DEGs of microglia, as shown in Table 2.
The sex-specific DEGs in oligodendrocyte
77,466 oligodendrocytic nuclei were analyzed (Figure 4A), with 42,469 from male AD (54.82%) and 34,997 from female AD (45.18%). Sex-specific DEGs revealed upregulation of 384 genes, including PCDH9, MT-CO1, NEAT1, and NPAS3, downregulation of 188 genes, including FRMD4A, PLP1 and LSAMP, and the rest 76,894 genes unchanged (Figure 4B). Further, GO and KEGG analyses identified that those DEGs primarily concentrated in the pathways of neurons, synapses, and hormones, with neuronal pathways including neuron spine, synaptic pathways including neuron-to-neuron synapse and glutamatergic/dopaminergic synapse, and hormone pathways including neurotrophin signaling pathway, aldosterone synthesis and secretion, calcium signaling pathway, etc (Figure 4C,D). Thirty genes with top frequency were obtained (Figure 4E), with GRIN2A and PSEN1 tied for second place. PPI networks were constructed to explore the relationship between these genes (Figure 4F) and identified GRIN2A and GRIA2 as core genes. UMAP plots displayed differences in selected DEGs: GRIN2A, ITPR2, GNAS, and XIST were higher in female AD and lower in male AD, while NLGN4Y, UTY, and TTTY14 were opposite (Figure 4G). GRIN2A, ITPR2, GNAS, and NLGN4Y were finally determined as sex-specific DEGs of oligodendrocytes, as shown in Table 3.
Interaction between key genes and the top 30 Genes of glial cells, and NLGN4Y as the common shared gene
The Venn diagrams and the PPI networks provided an overview of the close interaction between key genes (Figure 5A,B) and the top 30 genes (Figure 5C, D) of each glial cell. Results showed that ACYB, APP, JUN, PRKACB, and DLG2 were at the core of the PPI network, and NLGN4Y was a common shared gene for sex-specific DEGs in all glial cells.
Gene-TF-miRNA network construction
The NLGN4Y-TF-miRNA network contained 13 nodes and 12 edges (Figure 6A). NLGN4Y was regulated by 1 TF, namely CTCF, and 11 miRNAs, including hsa-miR-185, hsa-miR-137 and hsa-miR-9.
Displaying target drug and TCMs of NLGN4Y with network
A total of 1 NLGN4Y target drug and 64 indirect target TCMs were retrieved in Coremine Medical. TCMs with statistical significance in the results were marked with blue. Drug Antithrombin III and five TCMs with the network, namely Heikunbu, Wulingzhi, Xiazhicao, Shuizhi, and Mahuang, were visualized, which were considered statistically significant (Figure 6B).
Effects of target TCMs and corresponding active ingredients on AD
For Kunbu, 10 ingredients in TCMIP and 48 ingredients in TCMSP were retrieved. Through searching the PubMed database, 5 ingredients were retrieved related to AD: fucosterol, saringosterol, thiamine, stearidonic acid, and phlorofucofuroeckol-A, of which the oral bioavailability (OB) of the first two was ≥30% and similar to the drug sex (DL) was ≥0.18. Details are displayed in Table 4. As for Mahuang, 28 ingredients in TCMIP and 363 ingredients in TCMSP were retrieved. With the same method as Kunbu, 25 ingredients related to AD were retrieved. Among them, 6 ingredients with OB ≥30% and DL ≥0.18: quercetin, eriodictyol, naringenin, taxifolin, stigmasterol, and luteolin, are listed at the top of Table 5.
Hurb-gene-disease network and enrichment analysis
Hurb-gene-disease network is shown in Figure 6C. The shared target gene of Kunbu and Mahuang was ACHE, whose associated diseases were AD and cognitive deficits. The target genes of Kunbu alone were ALKBH3 and ELOVL4, diseases related to which were aging and brain atrophy, respectively.
The results of GO enrichments (BP, MF, and CC) for Kunbu (Figure 7A, Figure 8A, Figure 9A) and Mahuang (Figure 7B, Figure 8B, Figure 9B) are displayed with bar charts. Reactome pathways for Kunbu (Figure 10A) and Mahuang (Figure 10B) are also shown. The enriched terms marked with arrows were related to the "hormone-synapse-neuron" axis, such as steroid hormone receptor activity, neuron projection, and steroid hormone-mediated signaling pathway in Kunbu and chemical synaptic transmission, estrogen-dependent gene expression and nervous system process in Mahuang.
Figure 1: Gene expression data acquiring, single-nuclei RNA-seq profiling, and cell type characterization. (A) Samples obtained from GEO DataSets for analysis preparation. (B) 2-dimensional UMAP plot of sum nuclei (N = 116,101 for male; N = 103,994 for female). (C) Proportions for each type of cell split by gender. (D) Average expression of 5 well-established cell type markers projected on the UMAP plot. Please click here to view a larger version of this figure.
Figure 2: Astrocytes are heterogeneous and have sex-specific transcriptomic changes in Alzheimer's disease. (A) UMAP plot of astrocytic nuclei (N = 59,010). (B) Sex-specific DEGs. (C,D) Circle plots illustrated the significant functionally enriched terms of astrocytic DEGs obtained from GO and KEGG databases (GO: C, KEGG: D). (E) The top 30 most frequent astrocyte-sex DEGs in GO and KEGG pathways. (F) PPI network of the top 30 most frequent astrocyte-sex DEGs in GO and KEGG pathways. (G) Average expression of remarkable sex-specific DEGs projected on the UMAP plots. Please click here to view a larger version of this figure.
Figure 3: Microglia are heterogeneous and have sex-specific transcriptomic changes in Alzheimer's disease. (A) UMAP plot of microglial nuclei (N = 14,265). (B) Sex-specific DEGs. (C,D) Circle plots illustrated the significant functionally enriched terms of microglial DEGs obtained from GO and KEGG databases (GO: C, KEGG: D). (E) The top 30 most frequent microglia-sex DEGs inGO and KEGGpathways. (F) PPI network of the top 30 most frequent microglia-sex DEGs in GO and KEGG pathways. (G) Average expression of remarkable sex-specific DEGs projected on the UMAP plots. Please click here to view a larger version of this figure.
Figure 4: Oligodendrocytes are heterogeneous and have sex-specific transcriptomic changes in Alzheimer's disease. (A) UMAP plot of oligodendrocytic nuclei (N = 77,466). (B) Sex-specific DEGs. (C,D) Circle plots illustrated the significant functionally enriched terms of oligodendrocytic DEGs obtained from GO and KEGG databases (GO: C, KEGG: D). (E) The top 30 most frequent oligodendrocyte-sex DEGs in GO and KEGG pathways. (F) PPI network of the top 30 most frequent oligodendrocyte-sex DEGs in GO and KEGG pathways. (G) Average expression of remarkable sex-specific DEGs projected on the UMAP plots. Please click here to view a larger version of this figure.
Figure 5: Overlaps of DEGs and PPI networks of top frequency DEGs. (A,B) Venn diagram illustrating the key genes for each glia and the corresponding PPI network. (C,D) Venn diagram illustrating the top 30 frequent sex-specific DEGs for each glia enriched in GO and KEGG pathways and the corresponding PPI network. Please click here to view a larger version of this figure.
Figure 6: Network diagram with NLGN4Y and its targeting TCMs as core. (A) Gene-TF-miRNA coregulatory network. (B) Gene-drug-TCM network for NLGN4Y. (C) TCM-gene-disease network of Kunbu and Mahuang. Please click here to view a larger version of this figure.
Figure 7: GO (BP) Enrichment analysis for Kunbu and Mahuang. (A) Top 20 enriched biological processes of Kunbu. (B) Top 20 enriched biological processes of Mahuang. Please click here to view a larger version of this figure.
Figure 8: GO (MF) Enrichment analysis for Kunbu and Mahuang. (A) Top 20 enriched molecular functions of Kunbu. (B) Top 20 enriched molecular functions of Mahuang. Please click here to view a larger version of this figure.
Figure 9: GO (CC) Enrichment analysis for Kunbu and Mahuang. (A) Top 20 enriched cellular components of Kunbu. (B) Top 20 enriched cellular components of Mahuang. Please click here to view a larger version of this figure.
Figure 10: Reactome pathways for Kunbu and Mahuang. (A) Reactome pathways of Kunbu. (B) Reactome pathways of Mahuang. Please click here to view a larger version of this figure.
Table 1: Key genes of the sex-specific DEGs in astrocytes. Please click here to download this Table.
Table 2: Key genes of the sex-specific DEGs in microglia. Please click here to download this Table.
Table 3: Key genes of the sex-specific DEGs in oligodendrocytes. Please click here to download this Table.
Table 4: Kunbu' active ingredients on AD. Please click here to download this Table.
Table 5: Mahuang' active ingredients on AD. Please click here to download this Table.
Supplementary Figure 1: Screenshot for the R software usage. Please click here to download this File.
Supplementary Table 1: Sample information. Please click here to download this File.
Supplementary Table 2: Marker genes. Please click here to download this File.
Supplementary File 1: The R CODE. Please click here to download this File.
Gender-specificity has been identified in epidemiology, pathology, and clinical manifestation of AD19. Here, we confirmed the potential pathological mechanism of the “hormone-synapse-neuron axis” from gender-specific glial genes and related pathways in AD patients. NLGN4Y was the only shared gene in the three glia and was chosen as the biomarker for the gender specificity of AD. TF and miRNAs regulating NLGN4Y were strongly linked to gender differences and the development of the nervous system. Furthermore, the target TCMs Kunbu and Mahuang were considered to potentially affect the “hormone-synapse-neuron” axis and were identified to act as therapeutic candidates for AD by regulation of gender specificity.
The Harmony algorithm provided distinct advantages over other integration algorithms by integrating data in rare cells, optimizing memory usage and computational speed for large samples, and accommodating complex experimental designs with diverse cellular sources and technology platforms18. QC and data integration sections were critical components in enhancing the accuracy and reliability of the analysis, enabling researchers to glean more profound insights into the biology of AD and other neurodegenerative illnesses. The meticulous execution of these steps is pivotal in achieving the overall quality and validity of the results derived from single-nuclei RNA sequencing experiments.
One of the modifications made in this protocol was the use of the SCTransform function to normalize and standardize the data20. This step ensured that the data was comparable and standardized for further analysis. To mitigate the batch effect, an additional step of data integration was taken, which helped to correct the batch effect and improve the accuracy of the results. Troubleshooting was conducted when one of the samples (GSM5106107) showed unusual performance compared to the other samples, and it was excluded from the analysis.
One limitation of this study pertained to the relatively small sample size employed, which may restrict the representativeness of the findings to the broader population. Furthermore, the utilization of data from multiple laboratories and research groups introduced inherent heterogeneity, potentially limiting the reproducibility and generalizability of the results. Although the identification of key regulatory factors for NLGN4Y was achieved through a gene-TF-miRNA coregulatory network, further experimental verification was necessary to ascertain the functional roles and underlying mechanisms attributed to these regulatory factors. While enrichment analysis suggested Mahuang and Kunbu as potential candidates for gender-specific AD treatment, relying solely on bioinformatics predictions was insufficient to establish their efficacy and safety. Additional experiments and clinical studies were imperative to validate the therapeutic effects of these promising drugs.
The approach delineated in this study exhibited considerable potential for diverse research domains, notably in the discernment of sex-specific DEGs within glial cells in AD. Such investigations hold promise for elucidating the nuanced pathogenic disparities between male and female individuals, consequently facilitating the formulation of sex-specific therapeutic interventions. Moreover, the method’s applicability extended to other neurodegenerative conditions, offering opportunities to identify sex-specific DEGs and augment comprehension of the diseases’ underlying mechanisms.
In conclusion, the study presented a comprehensive and robust protocol for analyzing single-nuclei RNA sequencing data from AD patients, potentially paving the way for the development of tailored therapeutic interventions. Furthermore, the methodology employed in this study may be extended to other neurodegenerative conditions, offering opportunities to uncover sex-specific gene expression patterns and deepen the understanding of these complex diseases.
The authors have nothing to disclose.
The authors are grateful to Jessica S Sadick, Michael R O'Dea, Philip Hasel, etc., for providing the GSE167490 dataset. The authors appreciate that Faten A Sayed, Lay Kodama, Li Fan, etc., offer the GSE183068 dataset. The authors thank Shuqing Liu for the help with data analysis and Wen Yang for providing the data analysis platform. This study was supported by National Natural Science Foundation of China (82174511), Chengdu University of Traditional Chinese Medicine Apricot Grove Scholars, Discipline Talent Research Enhancement Program (QJJJ2022001), LiaoNing Revitalization Talents Program (XLYC 1807083), Sichuan Administration Bureau Fund of Chinese Medicine and Herbs (2023MS578), National Undergraduate Innovation and Entrepreneurship Training Project (202310633003X), and Innovative topics of scientific research practice for college students in Chengdu University of Traditional Chinese Medicine (ky-2023100). Hanjie Liu and Hui Yang contributed to the design of the study, collection, interpretation of data, and drafting, and revising the manuscript. Shuqing Liu and Siyu Li participated in the design of the study, collection of data and drafting the manuscript. Wen Yang and Anwar Ayesha were responsible for the collection and interpretation of data. Xin Tan prepared figures and/or tables. Cen Jiang, Yi Liu, and Lushuang Xie conceived the study and reviewed/edited the manuscript. All authors contributed to the article and approved the submitted version.
Database | |||
Coremine Medical database | Jointly developed by Norway, the Chinese Academy of Sciences, the Chinese Academy of Medical Sciences, the National Medical Library of the United States and other institutions | When you explore concepts in CoreMine Medical you access a database that is structured to relate important concepts, ranked by statistical relevance, to your topic. For example, if you type in "Alzheimer disease," in addition to retrieving documents and resources that discuss the disease, you will be able to view networks and lists that show how your query concept is related to other bio-medical concepts. This provides an overview of concepts that relate to your search as well as being an interface for navigating information on these concepts. Weblink: https://coremine.com/medical/ |
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Gene Expression Omnibus (GEO) | National Center for Biotechnology Information in the United States (NCBI) | GEO is a public functional genomics data repository supporting MIAME-compliant data submissions. Array- and sequence-based data are accepted. Tools are provided to help users query and download experiments and curated gene expression profiles. Weblink: https://www.ncbi.nlm.nih.gov/geo/ |
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Integrative Pharmacology-based Research Platform of Traditional Chinese Medicine (TCMIP, version: 2.0) | None | Introduction to the Integrated Pharmacology Based Network Computational Research Platform for Traditional Chinese Medicine [TCMIP v2.0], http://www.tcmip.cn/ ) It is an intelligent data mining platform based on the online database of the Encyclopedia of Traditional Chinese Medicine (ETCM), which integrates medical big data management and pharmacological computing services. It aims to reveal the scientific connotation of traditional Chinese medicine theory and the scientific value of original thinking in traditional Chinese medicine, summarize and pass on the experience of famous doctors, control the quality of traditional Chinese medicine, explain the principles of traditional Chinese medicine action, research and development of new Chinese medicine, especially the discovery and optimization of modern drug combinations, Provide a strong data foundation and analytical tools. Based on TCMIP v1.0, a comprehensive upgrade is implemented, including five major databases and seven functional modules. Through system integration and module integration, a comprehensive analysis of the multi-level correlation of the "disease syndrome prescription" interaction network can be quickly achieved. As an intelligent data mining platform, TCMIP v2.0 will provide a strong data foundation and analysis platform for revealing the scientific connotation of traditional Chinese medicine theory and the scientific value of original thinking in traditional Chinese medicine, summarizing and inheriting the experience of famous doctors, quality control of traditional Chinese medicine, elucidating the principles of traditional Chinese medicine action, research and development of new traditional Chinese medicine drugs, especially modern drug combination discovery and optimization. Weblink: http://www.tcmip.cn/TCMIP |
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NetworkAnalyst | None | Networkanalyze is an online visualization analysis platform for gene expression analysis and meta-analysis. It can perform comparative, quantitative, differential and enrichment analysis of gene expression, protein-protein interaction analysis, integration analysis of multiple datasets, and can also draw high-value images such as PCA, protein-protein interaction network diagram, heatmap, volcano diagram, Wayne diagram, etc. Weblink: https://www.networkanalyst.ca/NetworkAnalyst/ |
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PubMed database | National Center for Biotechnology Information in the United States (NCBI) | The Pubmed database is a biomedical literature database maintained by the National Library of Medicine (NLM) in the United States, aimed at providing the latest medical research results to scientists, doctors, researchers, and students worldwide. This database collects biomedical literature from around the world, including journal articles, papers, books, etc. As of now, the Pubmed database has collected over 30 million articles and is continuously updated every week. Weblink: https://pubmed.ncbi.nlm.nih.gov/ |
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R software | Ross Ihaka and Robert Gentleman | R is a language and environment for statistical computing and graphics. It is a GNU project which is similar to the S language and environment which was developed at Bell Laboratories (formerly AT&T, now Lucent Technologies) by John Chambers and colleagues. R can be considered as a different implementation of S. There are some important differences, but much code written for S runs unaltered under R. Weblink: https://www.r-project.org/ |
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STRING database (STRING, version 11.0) | Swiss Institute of Bioinformatics | STRING is a database of known and predicted protein interactions. The interactions include direct (physical) and indirect (functional) associations Weblink: https://string-db.org/ |
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Traditional Chinese Medicine Systems Pharmacology Database and Analysis Platform (TCMSP) | Zhejiang Jiuwei Health Co., Ltd | TCMSP is not only a data repository, but also an analysis platform for users to comprehensively study Traditional Chinese Medicines (TCM): including identification of active components, screening of drug targets and generation of compounds-targets-diseases networks, as well as the detailed drug pharmacokinetic information involving drug-likeness (DL), oral bioavailability (OB), blood-brain barrier (BBB),intestinal epithelial permeability (Caco-2), ALogP,fractional negative surface area (FASA-) and number of H-bond donor/acceptor (Hdon/Hacc). So far, TCMSP has attracted broad attentions and several groups have published more than 10 papers by using our TCMSP database within about one year. Weblink: https://tcmsp-e.com |