On‐Chip Neural Induction Boosts Neural Stem Cell Commitment: Toward a Pipeline for iPSC‐Based Therapies

Author:

Jain Saumey12ORCID,Voulgaris Dimitrios123ORCID,Thongkorn Surangrat24ORCID,Hesen Rick1ORCID,Hägg Alice5ORCID,Moslem Mohsen6ORCID,Falk Anna56ORCID,Herland Anna1236ORCID

Affiliation:

1. Division of Micro and Nanosystems KTH Royal Institute of Technology Malvinas väg 10 Stockholm 100 44 Sweden

2. Division of Nanobiotechnology Science for Life Laboratory KTH Royal Institute of Technology Tomtebodavägen 23a Solna 171 65 Sweden

3. AIMES Center for Integrated Medical and Engineering Science Department of Neuroscience Karolinska Institutet Solna 171 65 Sweden

4. Chulalongkorn Autism Research and Innovation Center of Excellence (Chula ACE) Department of Clinical Chemistry Faculty of Allied Health Sciences Chulalongkorn University Bangkok 10330 Thailand

5. Neural Stem Cells Department of Experimental Medical Science Lund Stem Cell Center Lund University Lund 221 84 Sweden

6. Department of Neuroscience Karolinska Institutet Solna 171 65 Sweden

Abstract

AbstractThe clinical translation of induced pluripotent stem cells (iPSCs) holds great potential for personalized therapeutics. However, one of the main obstacles is that the current workflow to generate iPSCs is expensive, time‐consuming, and requires standardization. A simplified and cost‐effective microfluidic approach is presented for reprogramming fibroblasts into iPSCs and their subsequent differentiation into neural stem cells (NSCs). This method exploits microphysiological technology, providing a 100‐fold reduction in reagents for reprogramming and a ninefold reduction in number of input cells. The iPSCs generated from microfluidic reprogramming of fibroblasts show upregulation of pluripotency markers and downregulation of fibroblast markers, on par with those reprogrammed in standard well‐conditions. The NSCs differentiated in microfluidic chips show upregulation of neuroectodermal markers (ZIC1, PAX6, SOX1), highlighting their propensity for nervous system development. Cells obtained on conventional well plates and microfluidic chips are compared for reprogramming and neural induction by bulk RNA sequencing. Pathway enrichment analysis of NSCs from chip showed neural stem cell development enrichment and boosted commitment to neural stem cell lineage in initial phases of neural induction, attributed to a confined environment in a microfluidic chip. This method provides a cost‐effective pipeline to reprogram and differentiate iPSCs for therapeutics compliant with current good manufacturing practices.

Funder

Lunds Universitet

Hjärnfonden

Royal Golden Jubilee (RGJ) Ph.D. Programme

Knut och Alice Wallenbergs Stiftelse

Vetenskapsrådet

Karolinska Institutet

Kungliga Tekniska Högskolan

Vinnova

Publisher

Wiley

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