Transcriptional complexity in the insect central complex: single nuclei RNA-sequencing of adult brain neurons derived from type 2 neuroblasts

Reviewer #1 (Public review):

Summary:

Epiney et al. use single-nuclei RNA sequencing (snRNA-seq) to characterize the lineage of Type-2 (T2) neuroblasts (NBs) in the adult Drosophila brain. To isolate cells born from T2 NBs, the authors used a genetic tool that specifically allows the permanent labeling of T2-derived cell types, which are then FAC-sorted for snRNA-seq. This effective labeling approach also allows them to compare the isolated T2 lineage cells with T1-derived cell types by a simple exclusion method. The authors begin by describing a transcriptomic atlas for all T1 and T2-derived neuronal and glia clusters, reporting that the T2-derived lineage comprises 161 neuronal clusters, in contrast to the T1 lineage which comprises 114 of them. The authors then use the expression of VAChT, VGlut, Gad1, Tbh, Ple, SerT, and Tdc2 to show that T2 neuroblasts generate all major neuron classes of fast-acting neurotransmitters. Strikingly, they show that a subset of glia and neuronal clusters have disproportionate enrichment in males or females, suggesting that T2 neuroblasts generate sex-biased cell types. The authors then proceed to characterize neuropeptide expression across T2-derived neuronal clusters and argue that the same neuropeptide can be expressed across different cell types, while similar cell types can express distinct neuropeptides. The functional implication of both observations, however, remains to be tested. Furthermore, the authors describe combinatorial transcription factor (TF) codes that are correlated with neuropeptide expression for T2-derived neurons along with an overall TF code for all T2-derived cell types, both of which will serve as an important starting point for future investigations. Finally, the authors map well-studied neuronal types of the central complex to the clusters of their T2-derived snRNA-seq dataset. They use known marker combinations, bulk RNA-seq data and highly specific split-GAL4 driver lines to annotate their T2-derived atlas, establishing a comprehensive transcriptomic atlas that would guide future studies in this field.

Strengths:

This study provides an in-depth transcriptomic characterization of neurons and glia derived from Type-2 neuroblast lineages. The results of this manuscript offer several future directions to investigate the mechanisms of diversifying neuronal identity. The datasets of T1-derived and T2-derived cells will pave the way for studies focused on the functional analysis of combinatorial TF codes specifying cell identity, sex-based differences in neurogenesis and gliogenesis, the relationship between neuropeptide (co)expression and cell identity, and the differential contributions of distinct progenitor populations to the same cell type.

Weaknesses:

The study presents several important observations based on the characterization of Type II neuroblast-derived lineages. However, a mechanistic insight is missing for most observations. The idea that there is a sex-specific bias to certain T2-derived neurons and glial clusters is quite interesting, however, the functional significance of this observation is not tested or discussed extensively. Finally, the authors do not show whether the combinatorial TF code is indeed necessary for neuropeptide expression or if this is just a correlation due to cell identity being defined by TFs. Functional knockdown of some candidate TFs for a subset of neuropeptide-expressing cells would have been helpful in this case.

Reviewer #2 (Public review):

In this manuscript, Epiney et al., present a single-nucleus sequencing analysis of Drosophila adult central brain neurons and glia. By employing an ingenious permanent labeling technique, they trace the progeny of T2 neuroblasts, which play a key role in the formation of the central complex. This transcriptomic dataset is poised to become a valuable resource for future research on neurogenesis, neuron morphology, and behavior.

The authors further delve into this dataset with several analyses, including the characterization of neurotransmitter expression profiles in T2-derived neurons. While some of the bioinformatic analyses are preliminary, they would benefit from additional experimental validation in future studies.