Peer review process
Not revised: This Reviewed Preprint includes the authors’ original preprint (without revision), an eLife assessment, public reviews, and a provisional response from the authors.
Read more about eLife’s peer review process.Editors
- Reviewing EditorMark SharpleyCedars-Sinai Medical Center, Los Angeles, United States of America
- Senior EditorUtpal BanerjeeUniversity of California, Los Angeles, Los Angeles, United States of America
Reviewer #1 (Public review):
Summary:
The study examines how pyruvate, a key product of glycolysis that influences TCA metabolism and gluconeogenesis, impacts cellular metabolism and cell size. It primarily utilizes the Drosophila liver-like fat body, which is composed of large post-mitotic cells that are metabolically very active. The study focuses on the key observations that over-expression of the pyruvate importer MPC complex (which imports pyruvate from the cytoplasm into mitochondria) can reduce cell size in a cell-autonomous manner. They find this is by metabolic rewiring that shunts pyruvate away from TCA metabolism and into gluconeogenesis. Surprisingly, mTORC and Myc pathways are also hyper-active in this background, despite the decreased cell size, suggesting a non-canonical cell size regulation signaling pathway. They also show a similar cell size reduction in HepG2 organoids. Metabolic analysis reveals that enhanced gluconeogenesis suppresses protein synthesis. Their working model is that elevated pyruvate mitochondrial import drives oxaloacetate production and fuels gluconeogenesis during late larval development, thus reducing amino acid production and thus reducing protein synthesis.
Strengths:
The study is significant because stem cells and many cancers exhibit metabolic rewiring of pyruvate metabolism. It provides new insights into how the fate of pyruvate can be tuned to influence Drosophila biomass accrual, and how pyruvate pools can influence the balance between carbohydrate and protein biosynthesis. Strengths include its rigorous dissection of metabolic rewiring and use of Drosophila and mammalian cell systems to dissect carbohydrate:protein crosstalk.
Weaknesses:
However, questions on how these two pathways crosstalk, and how this interfaces with canonical Myc and mTORC machinery remain. There are also questions related to how this protein:carbohydrate crosstalk interfaces with lipid biosynthesis. Addressing these will increase the overall impact of the study.
Reviewer #2 (Public review):
In this manuscript, the authors leverage multiple cellular models including the drosophila fat body and cultured hepatocytes to investigate the metabolic programs governing cell size. By profiling gene programs in the larval fat body during the third instar stage - in which cells cease proliferation and initiate a period of cell growth - the authors uncover a coordinated downregulation of genes involved in mitochondrial pyruvate import and metabolism. Enforced expression of the mitochondrial pyruvate carrier restrains cell size, despite active signaling of mTORC1 and other pathways viewed as traditional determinants of cell size. Mechanistically, the authors find that mitochondrial pyruvate import restrains cell size by fueling gluconeogenesis through the combined action of pyruvate carboxylase and phosphoenolpyruvate carboxykinase. Pyruvate conversion to oxaloacetate and use as a gluconeogenic substrate restrains cell growth by siphoning oxaloacetate away from aspartate and other amino acid biosynthesis, revealing a tradeoff between gluconeogenesis and provision of amino acids required to sustain protein biosynthesis. Overall, this manuscript is extremely rigorous, with each point interrogated through a variety of genetic and pharmacologic assays. The major conceptual advance is uncovering the regulation of cell size as a consequence of compartmentalized metabolism, which is dominant even over traditional signaling inputs. The work has implications for understanding cell size control in cell types that engage in gluconeogenesis but more broadly raise the possibility that metabolic tradeoffs determine cell size control in a variety of contexts.
Reviewer #3 (Public review):
Summary:
In this article, Toshniwal et al. investigate the role of pyruvate metabolism in controlling cell growth. They find that elevated expression of the mitochondrial pyruvate carrier (MPC) leads to decreased cell size in the Drosophila fat body, a transformed human hepatocyte cell line (HepG2), and primary rat hepatocytes. Using genetic approaches and metabolic assays, the authors find that elevated pyruvate import into cells with forced expression of MPC increases the cellular NADH/NAD+ ratio, which drives the production of oxaloacetate via pyruvate carboxylase. Genetic, pharmacological, and metabolic approaches suggest that oxaloacetate is used to support gluconeogenesis rather than amino acid synthesis in cells over-expressing MPC. The reduction in cellular amino acids impairs protein synthesis, leading to impaired cell growth.
Strengths:
This study shows that the metabolic program of a cell, and especially its NADH/NAD+ ratio, can play a dominant role in regulating cell growth.
The combination of complementary approaches, ranging from Drosophila genetics to metabolic flux measurements in mammalian cells, strengthens the findings of the paper and shows a conservation of MPC effects across evolution.
Weaknesses:
In general, the strengths of this paper outweigh its weaknesses. However, some areas of inconsistency and rigor deserve further attention.
The authors comment that MPC overrides hormonal controls on gluconeogenesis and cell size (Discussion, paragraph 3). Such a claim cannot be made for mammalian experiments that are conducted with immortalized cell lines or primary hepatocytes.
Nuclear size looks to be decreased in fat body cells with elevated MPC levels, consistent with reduced endoreplication, a process that drives growth in these cells. However, acute, ex vivo EdU labeling and measures of tissue DNA content are equivalent in wild-type and MPC+ fat body cells. This is surprising - how do the authors interpret these apparently contradictory phenotypes?
In Figure 4d, oxygen consumption rates are measured in control cells and those over-expressing MPC. Values are normalized to protein levels, but protein is reduced in MPC+ cells. Is oxygen consumption changed by MPC expression on a per-cell basis?
Trehalose is the main circulating sugar in Drosophila and should be measured in addition to hemolymph glucose. Additionally, the units in Figure 4h should be related to hemolymph volume - it is not clear that they are.
Measurements of NADH/NAD ratios in conditions where these are manipulated genetically and pharmacologically (Figure 5) would strengthen the findings of the paper. Along the same lines, expression of manipulated genes - whether by RT-qPCR or Western blotting - would be helpful to assess the degree of knockdown/knockout in a cell population (for example, Got2 manipulations in Figures 6 and S8).
Author response:
Reviewer #1 (Public review):
The study examines how pyruvate, a key product of glycolysis that influences TCA metabolism and gluconeogenesis, impacts cellular metabolism and cell size. It primarily utilizes the Drosophila liver-like fat body, which is composed of large post-mitotic cells that are metabolically very active. The study focuses on the key observations that over-expression of the pyruvate importer MPC complex (which imports pyruvate from the cytoplasm into mitochondria) can reduce cell size in a cell-autonomous manner. They find this is by metabolic rewiring that shunts pyruvate away from TCA metabolism and into gluconeogenesis. Surprisingly, mTORC and Myc pathways are also hyper-active in this background, despite the decreased cell size, suggesting a non-canonical cell size regulation signaling pathway. They also show a similar cell size reduction in HepG2 organoids. Metabolic analysis reveals that enhanced gluconeogenesis suppresses protein synthesis. Their working model is that elevated pyruvate mitochondrial import drives oxaloacetate production and fuels gluconeogenesis during late larval development, thus reducing amino acid production and thus reducing protein synthesis.
Strengths:
The study is significant because stem cells and many cancers exhibit metabolic rewiring of pyruvate metabolism. It provides new insights into how the fate of pyruvate can be tuned to influence Drosophila biomass accrual, and how pyruvate pools can influence the balance between carbohydrate and protein biosynthesis. Strengths include its rigorous dissection of metabolic rewiring and use of Drosophila and mammalian cell systems to dissect carbohydrate:protein crosstalk.
Weaknesses:
However, questions on how these two pathways crosstalk, and how this interfaces with canonical Myc and mTORC machinery remain. There are also questions related to how this protein:carbohydrate crosstalk interfaces with lipid biosynthesis. Addressing these will increase the overall impact of the study.
We thank the reviewer for recognizing the significance of our work and for providing constructive feedback. Our findings indicate that elevated pyruvate transport into mitochondria acts independently of canonical pathways, such as mTORC1 or Myc signaling, to regulate cell size. To investigate these pathways, we utilized immunofluorescence with well-validated surrogate measures (p-S6 and p-4EBP1) in clonal analyses of MPC expression, as well as RNA-seq analyses in whole fat body tissues expressing MPC. These methods revealed hyperactivation of mTORC1 and Myc signaling in fat body cells expressing MPC in Drosophila, which are dramatically smaller than control cells. One explanation of these seemingly contradictory observations could be an excess of nutrients that activate mTORC1 or Myc pathways. However, our data is inconsistent with a nutrient surplus that could explain this hyperactivation. Instead, we observed reduced amino acid abundance upon MPC expression, which is very surprising given the observed hyperactivation of mTORC1. This led us to hypothesize the existence of a feedback mechanism that senses inappropriate reductions in cell size and activates signaling pathways to promote cell growth. The best characterized “sizer” pathway for mammalian cells is the CycD/CDK4 complex which has been well studied in the context of cell size regulation of the cell cycle (PMID 10970848, 34022133). However, the mechanisms that sense cell size in post-mitotic cells, such as fat body cells and hepatocytes, remain poorly understood. Investigating the hypothesized size-sensing mechanisms at play here is a fascinating direction for future research.
For the current study, we conducted epistatic analyses with mTOR pathway members by overexpressing PI3K and knocking down the TORC1 inhibitor Tuberous Sclerosis Complex 1 (Tsc1). These manipulations increased the size of control fat body cells but not those over-expressing the MPC (Supplementary Fig. 3c, 3d). Regarding Myc, its overexpression increased the size of both control and MPC+ clones (Supplementary Fig. 3e), but Myc knockdown had no additional effect on cell size in MPC+ clones (Supplementary Fig. 3f). These results suggest that neither mTORC1, PI3K, nor Myc are epistatic to the cell size effects of MPC expression. Consequently, we shifted our focus to metabolic mechanisms regulating biomass production and cell size.
When analyzing cellular biomolecules contributing to biomass, we observed a significant impact on protein levels in Drosophila fat body cells and mammalian MPC-expressing HepG2 spheroids. TAG abundance in MPC-expressing HepG2 spheroids and whole fat body cells showed a statistically insignificant decrease compared to controls. Furthermore, lipid droplets in fat body cells were comparable in MPC-expressing clones when normalized to cell size.
Interestingly, RNA-seq analysis revealed increased expression of fatty acid and cholesterol biosynthesis pathways in MPC-expressing fat body cells. Upregulated genes included major SREBP targets, such as ATPCL (2.08-fold), FASN1 (1.15-fold), FASN2 (1.07-fold), and ACC (1.26-fold). Since mTOR promotes SREBP activation and MPC-expressing cells showed elevated mTOR activity and upregulation of SREBP targets, we hypothesize that SREBP is activated in these cells. Nonetheless, our data on amino acid abundance and its impact on protein synthesis activity suggest that protein abundance, rather than lipids, is likely to play a larger causal role in regulating cell size in response to increased pyruvate transport into mitochondria.
Reviewer #2 (Public review):
In this manuscript, the authors leverage multiple cellular models including the drosophila fat body and cultured hepatocytes to investigate the metabolic programs governing cell size. By profiling gene programs in the larval fat body during the third instar stage - in which cells cease proliferation and initiate a period of cell growth - the authors uncover a coordinated downregulation of genes involved in mitochondrial pyruvate import and metabolism. Enforced expression of the mitochondrial pyruvate carrier restrains cell size, despite active signaling of mTORC1 and other pathways viewed as traditional determinants of cell size. Mechanistically, the authors find that mitochondrial pyruvate import restrains cell size by fueling gluconeogenesis through the combined action of pyruvate carboxylase and phosphoenolpyruvate carboxykinase. Pyruvate conversion to oxaloacetate and use as a gluconeogenic substrate restrains cell growth by siphoning oxaloacetate away from aspartate and other amino acid biosynthesis, revealing a tradeoff between gluconeogenesis and provision of amino acids required to sustain protein biosynthesis. Overall, this manuscript is extremely rigorous, with each point interrogated through a variety of genetic and pharmacologic assays. The major conceptual advance is uncovering the regulation of cell size as a consequence of compartmentalized metabolism, which is dominant even over traditional signaling inputs. The work has implications for understanding cell size control in cell types that engage in gluconeogenesis but more broadly raise the possibility that metabolic tradeoffs determine cell size control in a variety of contexts.
We thank the reviewer for their thoughtful recognition of our efforts, and we are honored by the enthusiasm the reviewer expressed for the findings and the significance of our research. We share the reviewer’s opinion that our work might help to unravel metabolic mechanisms that regulate biomass gain independent of the well-known signaling pathways.
Reviewer #3 (Public review):
Summary:
In this article, Toshniwal et al. investigate the role of pyruvate metabolism in controlling cell growth. They find that elevated expression of the mitochondrial pyruvate carrier (MPC) leads to decreased cell size in the Drosophila fat body, a transformed human hepatocyte cell line (HepG2), and primary rat hepatocytes. Using genetic approaches and metabolic assays, the authors find that elevated pyruvate import into cells with forced expression of MPC increases the cellular NADH/NAD+ ratio, which drives the production of oxaloacetate via pyruvate carboxylase. Genetic, pharmacological, and metabolic approaches suggest that oxaloacetate is used to support gluconeogenesis rather than amino acid synthesis in cells over-expressing MPC. The reduction in cellular amino acids impairs protein synthesis, leading to impaired cell growth.
Strengths:
This study shows that the metabolic program of a cell, and especially its NADH/NAD+ ratio, can play a dominant role in regulating cell growth.
The combination of complementary approaches, ranging from Drosophila genetics to metabolic flux measurements in mammalian cells, strengthens the findings of the paper and shows a conservation of MPC effects across evolution.
Weaknesses:
In general, the strengths of this paper outweigh its weaknesses. However, some areas of inconsistency and rigor deserve further attention.
Thank you for reviewing our manuscript and offering constructive feedback. We appreciate your recognition of the significance of our work and your acknowledgment of the compelling evidence we have presented. We will carefully revise the manuscript in line with the reviewers' recommendations.
The authors comment that MPC overrides hormonal controls on gluconeogenesis and cell size (Discussion, paragraph 3). Such a claim cannot be made for mammalian experiments that are conducted with immortalized cell lines or primary hepatocytes.
We appreciate the reviewer’s insightful comment. Pyruvate is a primary substrate for gluconeogenesis, and our findings suggest that increased pyruvate transport into mitochondria increases the NADH-to-NAD+ ratio, and thereby elevates gluconeogenesis. Notably, we did not observe any changes in the expression of key glucagon targets, such as PC, PEPCK2, and G6PC, suggesting that the glucagon response is not activated upon MPC expression. By the statement referenced by the reviewer, we intended to highlight that excess pyruvate import into mitochondria drives gluconeogenesis independently of hormonal and physiological regulation.
It seems the reviewer might also have been expressing the sentiment that our in vitro models may not fully reflect the in vivo situation, and we completely agree. Moving forward, we plan to perform similar analyses in mammalian models to test the in vivo relevance of this mechanism. For now, we will refine the language in the manuscript to clarify this point.
Nuclear size looks to be decreased in fat body cells with elevated MPC levels, consistent with reduced endoreplication, a process that drives growth in these cells. However, acute, ex vivo EdU labeling and measures of tissue DNA content are equivalent in wild-type and MPC+ fat body cells. This is surprising - how do the authors interpret these apparently contradictory phenotypes?
We thank the reviewer for raising this important issue. The size of the nucleus is regulated by DNA content and various factors, including the physical properties of DNA, chromatin condensation, the nuclear lamina, and other structural components (PMID 32997613). Additionally, cytoplasmic and cellular volume also impacts nuclear size, as extensively documented during development (PMID 17998401, PMID 32473090).
In MPC-expressing cells, it is plausible that the reduced cellular volume impacts chromatin condensation or the nuclear lamina in a way that slightly decreases nuclear size without altering DNA content. Specifically, in our whole fat body experiments using CG-Gal4 (as shown in Supplementary Figure 2a-c), we noted that after 12 hours of MPC expression, cell size was significantly reduced (Supplementary Figure 2c and Author response image 1A). However, the reduction in nuclear size became significant only after 36 hours of MPC expression (Author response image 1B), suggesting that the reduction in cell size is a more acute response to MPC expression, followed only later by effects on nuclear size.
In clonal analyses, this relationship was further clarified. MPC-expressing cells with a size greater than 1000 µm² displayed nuclear sizes comparable to control cells, whereas those with a drastic reduction in cell size (less than 1000 µm²) exhibited smaller nuclei (Author response image 1C and D). These observations collectively suggest that changes in nuclear size are more likely to be downstream rather than upstream of cell size reduction. Given that DNA content remains unaffected, we focused on investigating the rate of protein synthesis. Our findings suggest that protein synthesis might play a causal role in regulating cell size, thereby reinforcing the connection between cellular and nuclear size in this context.
Author response image 1.
Cell Size vs. Nuclear Size in MPC-Expressing Fat Body Cells. A. Cell size comparison between control (blue, ay-GFP) and MPC+ (red, ay-MPC) fat body cells over time, measured in hours after MPC expression induction. B. Nuclear area measurements from the same fat body cells in ay-GFP and ay-MPC groups. C. Scatter plot of nuclear area vs. cell area for control (ay-GFP) cells, including the corresponding R² value. D. Scatter plot of nuclear area vs. cell area for MPC-expressing (ay-MPC) cells, with the respective R² value.
This image highlights the relationship between nuclear and cell size in MPC-expressing fat body cells, emphasizing the distinct cellular responses observed following MPC induction.
In Figure 4d, oxygen consumption rates are measured in control cells and those over-expressing MPC. Values are normalized to protein levels, but protein is reduced in MPC+ cells. Is oxygen consumption changed by MPC expression on a per-cell basis?
As described in the manuscript, MPC-expressing cells are smaller in size. In this context, we felt that it was most appropriate to normalize oxygen consumption rates (OCR) to cellular mass to enable an accurate interpretation of metabolic activity. Therefore, we normalized OCR with protein content to account for variations in cellular size and (probably) mitochondrial mass.
Trehalose is the main circulating sugar in Drosophila and should be measured in addition to hemolymph glucose. Additionally, the units in Figure 4h should be related to hemolymph volume - it is not clear that they are.
We appreciate this valuable suggestion. In the revised manuscript, we will quantify trehalose abundance in circulation and within fat bodies. As described in the Methods section, following the approach outlined in Ugrankar-Banerjee et al., 2023, we bled 10 larvae (either control or MPC-expressing) using forceps onto parafilm. From this, 2 microliters of hemolymph were collected for glucose measurement. We will apply this methodology to include the trehalose measurements as part of our updated analysis.
Measurements of NADH/NAD ratios in conditions where these are manipulated genetically and pharmacologically (Figure 5) would strengthen the findings of the paper. Along the same lines, expression of manipulated genes - whether by RT-qPCR or Western blotting - would be helpful to assess the degree of knockdown/knockout in a cell population (for example, Got2 manipulations in Figures 6 and S8).
We appreciate this suggestion, which will provide additional rigor to our study. We have already quantified NADH/NAD+ ratios in HepG2 cells under UK5099, NMN, and Asp supplementation, as presented in Figure 6k. As suggested, we will quantify the expression of Got2 manipulations mentioned in Figure 6j using RT-qPCR and validate the corresponding data in Supplementary Figure 8f through western blot analysis.
Additionally, we will assess the efficiency of pcb, pdha, dlat, pepck2, and Got2 manipulations used to modulate the expression of these genes. These validations will ensure the robustness of our findings and strengthen the conclusions of our study.
