Last updated: 2020-12-10
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library(tidyverse)
library(GGally)
library(gridExtra)
library(ggridges)
library(brms)
library(tidybayes)
library(DT)
library(kableExtra)
library(knitrhooks) # install with devtools::install_github("nathaneastwood/knitrhooks")
output_max_height() # a knitrhook option
options(stringsAsFactors = FALSE)
This analysis set out to test whether sexual selection treatment had an effect on metabolite composition of flies. We measured fresh and dry fly weight in milligrams, plus the weights of five metabolites which together equal the dry weight. These are:
Lipid_conc
(i.e. the weight of the hexane fraction, divided by the full dry weight),Carbohydrate_conc
(i.e. the weight of the aqueous fraction, divided by the full dry weight),Protein_conc
(i.e. \(\mu\)g of protein per milligram as measured by the bicinchoninic acid protein assay),Glycogen_conc
(i.e. \(\mu\)g of glycogen per milligram as measured by the hexokinase assay), andChitin_conc
(estimated as the difference between the initial and final dry weights)We expect body weight to vary between the sexes and potentially between treatments. In turn, we expect body weight to affect our five response variables of interest. Larger flies will have more lipids, carbs, etc., and this may vary by sex and treatment both directly and indirectly.
metabolites <- read_csv('data/3.metabolite_data.csv') %>%
mutate(sex = ifelse(sex == "m", "Male", "Female"),
line = paste(treatment, line, sep = ""),
treatment = ifelse(treatment == "M", "Monogamy", "Polyandry")) %>%
# log transform glycogen since it shows a long tail (others are reasonably normal-looking)
mutate(Glycogen_ug_mg = log(Glycogen_ug_mg)) %>%
# There was a technical error with flies collected on day 1,
# so they are excluded from the whole paper. All the measurements analysed are of 3d-old flies
filter(time == '2') %>%
select(-time)
scaled_metabolites <- metabolites %>%
# Find proportional metabolites as a proportion of total dry weight
mutate(
Dry_weight = dwt_mg,
Lipid_conc = Hex_frac / Dry_weight,
Carbohydrate_conc = Aq_frac / Dry_weight,
Protein_conc = Protein_ug_mg,
Glycogen_conc = Glycogen_ug_mg,
Chitin_conc = Chitin_mg_mg) %>%
select(sex, treatment, line, Dry_weight, ends_with("conc")) %>%
mutate_at(vars(ends_with("conc")), ~ as.numeric(scale(.x))) %>%
mutate(Dry_weight = as.numeric(scale(Dry_weight))) %>%
mutate(sextreat = paste(sex, treatment),
sextreat = replace(sextreat, sextreat == "Male Monogamy", "M males"),
sextreat = replace(sextreat, sextreat == "Male Polyandry", "P males"),
sextreat = replace(sextreat, sextreat == "Female Monogamy", "M females"),
sextreat = replace(sextreat, sextreat == "Female Polyandry", "P females"),
sextreat = factor(sextreat, c("M males", "P males", "M females", "P females")))
All variables are shown in standard units (i.e. mean = 0, SD = 1).
my_data_table <- function(df){
datatable(
df, rownames=FALSE,
autoHideNavigation = TRUE,
extensions = c("Scroller", "Buttons"),
options = list(
dom = 'Bfrtip',
deferRender=TRUE,
scrollX=TRUE, scrollY=400,
scrollCollapse=TRUE,
buttons =
list('csv', list(
extend = 'pdf',
pageSize = 'A4',
orientation = 'landscape',
filename = 'Apis_methylation')),
pageLength = 50
)
)
}
scaled_metabolites %>%
select(-sextreat) %>%
mutate_if(is.numeric, ~ format(round(.x, 3), nsmall = 3)) %>%
my_data_table()
The following plot shows how each metabolite varies between sexes and treatments, and how the consecration of each metabolite co-varies with dry weight across individuals.
levels <- c("Carbohydrate", "Chitin", "Glycogen", "Lipid", "Protein", "Dryweight")
cols <- c("M females" = "pink",
"P females" = "red",
"M males" = "skyblue",
"P males" = "blue")
grid.arrange(
scaled_metabolites %>%
rename_all(~ str_remove_all(.x, "_conc")) %>%
mutate(sex = factor(sex, c("Male", "Female"))) %>%
reshape2::melt(id.vars = c('sex', 'treatment', 'sextreat', 'line', 'Dry_weight')) %>%
mutate(variable = factor(variable, levels)) %>%
ggplot(aes(x = sex, y = value, fill = sextreat)) +
geom_hline(yintercept = 0, linetype = 2) +
geom_boxplot() +
facet_grid( ~ variable) +
theme_bw() +
xlab("Sex") + ylab("Concentration") +
theme(legend.position = 'top') +
scale_fill_manual(values = cols, name = ""),
scaled_metabolites %>%
rename_all(~ str_remove_all(.x, "_conc")) %>%
reshape2::melt(id.vars = c('sex', 'treatment', 'sextreat', 'line', 'Dry_weight')) %>%
mutate(variable = factor(variable, levels)) %>%
ggplot(aes(x = Dry_weight, y = value, colour = sextreat, fill = sextreat)) +
geom_smooth(method = 'lm', se = TRUE, aes(colour = NULL, fill = NULL), colour = "grey20", size = .4) +
geom_point(pch = 21, colour = "grey20") +
facet_grid( ~ variable) +
theme_bw() +
xlab("Dry weight") + ylab("Concentration") +
theme(legend.position = 'none') +
scale_colour_manual(values = cols, name = "") +
scale_fill_manual(values = cols, name = ""),
heights = c(0.55, 0.45)
)
Some of the metabolites, especially lipid concentration, are correlated with dry weight. There is also a large difference in dry weight between sexes (and treatments, to a less extent), and sex and treatment effects are evident for some of the metabolites in the raw data. Some of the metabolites are weakly correlated with other metabolites, e.g. lipid and glycogen concentration.
modified_densityDiag <- function(data, mapping, ...) {
ggally_densityDiag(data, mapping, colour = "grey10", ...) +
scale_fill_manual(values = cols) +
scale_x_continuous(guide = guide_axis(check.overlap = TRUE))
}
modified_points <- function(data, mapping, ...) {
ggally_points(data, mapping, pch = 21, colour = "grey10", ...) +
scale_fill_manual(values = cols) +
scale_x_continuous(guide = guide_axis(check.overlap = TRUE))
}
modified_facetdensity <- function(data, mapping, ...) {
ggally_facetdensity(data, mapping, ...) +
scale_colour_manual(values = cols)
}
modified_box_no_facet <- function(data, mapping, ...) {
ggally_box_no_facet(data, mapping, colour = "grey10", ...) +
scale_fill_manual(values = cols)
}
pairs_plot <- scaled_metabolites %>%
arrange(sex, treatment) %>%
select(-line, -sex, -treatment) %>%
rename(`Sex and treatment` = sextreat) %>%
rename_all(~ str_replace_all(.x, "_", " ")) %>%
ggpairs(aes(colour = `Sex and treatment`, fill = `Sex and treatment`),
diag = list(continuous = wrap(modified_densityDiag, alpha = 0.7),
discrete = wrap("blank")),
lower = list(continuous = wrap(modified_points, alpha = 0.7, size = 1.1),
discrete = wrap("blank"),
combo = wrap(modified_box_no_facet, alpha = 0.7)),
upper = list(continuous = wrap(modified_points, alpha = 0.7, size = 1.1),
discrete = wrap("blank"),
combo = wrap(modified_box_no_facet, alpha = 0.7, size = 0.5)))
pairs_plot
Version | Author | Date |
---|---|---|
43cc270 | lukeholman | 2020-12-09 |
se <- function(x) sd(x) / sqrt(length(x))
metabolites %>%
group_by(sex, treatment) %>%
summarise(mean_dwt = mean(dwt_mg),
SE = se(dwt_mg),
n = n()) %>%
kable(digits = 3) %>% kable_styling(full_width = FALSE)
sex | treatment | mean_dwt | SE | n |
---|---|---|---|---|
Female | Monogamy | 0.562 | 0.019 | 12 |
Female | Polyandry | 0.644 | 0.017 | 12 |
Male | Monogamy | 0.330 | 0.009 | 12 |
Male | Polyandry | 0.353 | 0.009 | 12 |
This directed acyclic graph (DAG) illustrates the causal pathways that we observed between the experimental or measured variables (square boxes) and latent variables (ovals). We hypothesise that sex and mating system potentially influence dry weight as well as the metabolite composition (which we assessed by estimating the concentrations of carbohydrates, chitin, glycogen, lipids and protein). Additionally, dry weight is likely correlated with metabolite composition, and so dry weight acts as a ‘mediator variable’ between metabolite composition, and sex and treatment. The structural equation model below is built with this DAG in mind.
DiagrammeR::grViz('digraph {
graph [layout = dot, rankdir = LR]
# define the global styles of the nodes. We can override these in box if we wish
node [shape = rectangle, style = filled, fillcolor = Linen]
"Metabolite\ncomposition" [shape = oval, fillcolor = Beige]
# edge definitions with the node IDs
"Mating system\ntreatment (M vs P)" -> {"Dry weight"}
"Mating system\ntreatment (M vs P)" -> {"Metabolite\ncomposition"}
"Sex\n(Female vs Male)" -> {"Dry weight"} -> {"Metabolite\ncomposition"}
"Sex\n(Female vs Male)" -> {"Metabolite\ncomposition"}
{"Metabolite\ncomposition"} -> "Carbohydrates"
{"Metabolite\ncomposition"} -> "Chitin"
{"Metabolite\ncomposition"} -> "Glycogen"
{"Metabolite\ncomposition"} -> "Lipids"
{"Metabolite\ncomposition"} -> "Protein"
}')
brms
structural equation modelHere we fit a model of the five metabolites, which includes dry body weight as a mediator variable. That is, our model estimates the effect of treatment, sex and line (and all the 2- and 3-way interactions) on dry weight, and then estimates the effect of those some predictors (plus dry weight) on the five metabolites. The model assumes that although the different sexes, treatment groups, and lines may differ in their dry weight, the relationship between dry weight and the metabolites does not vary by sex/treatment/line. This assumption was made to constrain the number of parameters in the model, and to reflect out prior beliefs about allometric scaling of metabolites.
We use set Normal
priors on all fixed effect parameters, mean = 0, sd = 1, which ‘regularises’ the estimates towards zero – this is conservative (because it makes large posterior effect sizes more improbable), and it also helps the model to converge. Similarly, we set a somewhat conservative half-cauchy prior (mean 0, scale 0.01) on the random effects for line
(i.e. we consider large differences between lines – in terms of means and treatment effects – to be possible but improbable). We leave all other priors at the defaults used by brms
.
prior1 <- c(set_prior("normal(0, 0.5)", class = "b", resp = 'Lipid'),
set_prior("normal(0, 0.5)", class = "b", resp = 'Carbohydrate'),
set_prior("normal(0, 0.5)", class = "b", resp = 'Protein'),
set_prior("normal(0, 0.5)", class = "b", resp = 'Glycogen'),
set_prior("normal(0, 0.5)", class = "b", resp = 'Chitin'),
set_prior("normal(0, 1)", class = "b", resp = 'Dryweight'),
set_prior("cauchy(0, 0.01)", class = "sd", resp = 'Lipid', group = "line"),
set_prior("cauchy(0, 0.01)", class = "sd", resp = 'Carbohydrate', group = "line"),
set_prior("cauchy(0, 0.01)", class = "sd", resp = 'Protein', group = "line"),
set_prior("cauchy(0, 0.01)", class = "sd", resp = 'Glycogen', group = "line"),
set_prior("cauchy(0, 0.01)", class = "sd", resp = 'Chitin', group = "line"),
set_prior("cauchy(0, 0.01)", class = "sd", resp = 'Dryweight', group = "line"))
prior1
prior class coef group resp dpar nlpar bound source normal(0, 0.5) b Lipid user normal(0, 0.5) b Carbohydrate user normal(0, 0.5) b Protein user normal(0, 0.5) b Glycogen user normal(0, 0.5) b Chitin user normal(0, 1) b Dryweight user cauchy(0, 0.01) sd line Lipid user cauchy(0, 0.01) sd line Carbohydrate user cauchy(0, 0.01) sd line Protein user cauchy(0, 0.01) sd line Glycogen user cauchy(0, 0.01) sd line Chitin user cauchy(0, 0.01) sd line Dryweight user
The fixed effects formula is sex * treatment + Dryweight
(or sex * treatment
in the case of the model of dry weight). The random effects part of the formula indicates that the 8 independent selection lines may differ in their means, and that the treatment effect may vary in sign/magnitude between lines. The notation | p |
means that the model estimates the correlations in line effects (both slopes and intercepts) between the 6 response variables. Finally, the notation set_rescor(TRUE)
means that the model should estimate the residual correlations between the response variables.
brms_formula <-
# Sub-models of the 5 metabolites
bf(mvbind(Lipid, Carbohydrate, Protein, Glycogen, Chitin) ~
sex*treatment + Dryweight + (treatment | p | line)) +
# dry weight sub-model
bf(Dryweight ~ sex*treatment + (treatment | p | line)) +
# Allow for (and estimate) covariance between the residuals of the difference response variables
set_rescor(TRUE)
brms_formula
Lipid ~ sex * treatment + Dryweight + (treatment | p | line) Carbohydrate ~ sex * treatment + Dryweight + (treatment | p | line) Protein ~ sex * treatment + Dryweight + (treatment | p | line) Glycogen ~ sex * treatment + Dryweight + (treatment | p | line) Chitin ~ sex * treatment + Dryweight + (treatment | p | line) Dryweight ~ sex * treatment + (treatment | p | line)
The model is run over 4 chains with 5000 iterations each (with the first 2500 discarded as burn-in), for a total of 2500*4 = 10,000 posterior samples.
if(!file.exists("output/brms_metabolite_SEM.rds")){
brms_metabolite_SEM <- brm(
brms_formula,
data = scaled_metabolites %>% # brms does not like underscores in variable names
rename(Dryweight = Dry_weight) %>%
rename_all(~ gsub("_conc", "", .x)),
iter = 5000, chains = 4, cores = 1,
prior = prior1,
control = list(max_treedepth = 20,
adapt_delta = 0.99)
)
saveRDS(brms_metabolite_SEM, "output/brms_metabolite_SEM.rds")
} else {
brms_metabolite_SEM <- readRDS('output/brms_metabolite_SEM.rds')
}
The plot below shows that the fitted model is able to produce posterior predictions that have a similar distribution to the original data, for each of the response variables, which is a necessary condition for the model to be used for statistical inference.
grid.arrange(
pp_check(brms_metabolite_SEM, resp = "Dryweight") +
ggtitle("Dry weight") + theme(legend.position = "none"),
pp_check(brms_metabolite_SEM, resp = "Lipid") +
ggtitle("Lipid") + theme(legend.position = "none"),
pp_check(brms_metabolite_SEM, resp = "Carbohydrate") +
ggtitle("Carbohydrate") + theme(legend.position = "none"),
pp_check(brms_metabolite_SEM, resp = "Protein") +
ggtitle("Protein") + theme(legend.position = "none"),
pp_check(brms_metabolite_SEM, resp = "Glycogen") +
ggtitle("Glycogen") + theme(legend.position = "none"),
pp_check(brms_metabolite_SEM, resp = "Chitin") +
ggtitle("Chitin") + theme(legend.position = "none"),
nrow = 1
)
Version | Author | Date |
---|---|---|
f7c88a2 | lukeholman | 2020-12-10 |
This tables shows the fixed effects estimates for the treatment, sex, their interaction, as well as the slope associated with dry weight (where relevant), for each of the six response variables. The p
column shows 1 - minus the “probability of direction”, i.e. the posterior probability that the reported sign of the estimate is correct given the data and the prior; subtracting this value from one gives a Bayesian equivalent of a one-sided p-value. For brevity, we have omitted all the parameter estimates involving the predictor variable line
, as well as the estimates of residual (co)variance. Click the next tab to see a complete summary of the model and its output.
vars <- c("Lipid", "Carbohydrate", "Glycogen", "Protein", "Chitin")
tests <- c('_Dryweight', '_sexMale',
'_sexMale:treatmentPolyandry',
'_treatmentPolyandry')
hypSEM <- data.frame(expand_grid(vars, tests) %>%
mutate(est = NA,
err = NA,
lwr = NA,
upr = NA) %>%
# bind body weight on the end
rbind(data.frame(
vars = rep('Dryweight', 3),
tests = c('_sexMale',
'_treatmentPolyandry',
'_sexMale:treatmentPolyandry'),
est = NA,
err = NA,
lwr = NA,
upr = NA)))
for(i in 1:nrow(hypSEM)) {
result = hypothesis(brms_metabolite_SEM,
paste0(hypSEM[i, 1], hypSEM[i, 2], ' = 0'))$hypothesis
hypSEM[i, 3] = round(result$Estimate, 3)
hypSEM[i, 4] = round(result$Est.Error, 3)
hypSEM[i, 5] = round(result$CI.Lower, 3)
hypSEM[i, 6] = round(result$CI.Upper, 3)
}
pvals <- bayestestR::p_direction(brms_metabolite_SEM) %>%
as.data.frame() %>%
mutate(vars = map_chr(str_split(Parameter, "_"), ~ .x[2]),
tests = map_chr(str_split(Parameter, "_"), ~ .x[3]),
tests = str_c("_", str_remove_all(tests, "[.]")),
tests = replace(tests, tests == "_sexMaletreatmentPolyandry", "_sexMale:treatmentPolyandry")) %>%
filter(!str_detect(tests, "line")) %>%
mutate(p_val = 1 - pd, star = ifelse(p_val < 0.05, "*", "")) %>%
select(vars, tests, p_val, star)
hypSEM <- hypSEM %>% left_join(pvals, by = c("vars", "tests"))
hypSEM %>%
mutate(Parameter = c(rep(c('Dry weight', 'Sex (M)',
'Sex (M) x Treatment (P)',
'Treatment (P)'), 5),
'Sex (M)', 'Treatment (P)', 'Sex (M) x Treatment (P)')) %>%
mutate(Parameter = factor(Parameter, c("Dry weight", "Sex (M)", "Treatment (P)", "Sex (M) x Treatment (P)")),
vars = factor(vars, c("Carbohydrate", "Chitin", "Glycogen", "Lipid", "Protein", "Dryweight"))) %>%
arrange(vars, Parameter) %>%
select(Parameter, Estimate = est, `Est. error` = err,
`CI lower` = lwr, `CI upper` = upr, `p` = p_val, star) %>%
rename(` ` = star) %>%
kable() %>%
kable_styling(full_width = FALSE) %>%
group_rows("Carbohydrates", 1, 4) %>%
group_rows("Chitin", 5, 8) %>%
group_rows("Glycogen", 9, 12) %>%
group_rows("Lipids", 13, 16) %>%
group_rows("Protein", 17, 20) %>%
group_rows("Dry weight", 21, 23)
Parameter | Estimate | Est. error | CI lower | CI upper | p | |
---|---|---|---|---|---|---|
Carbohydrates | ||||||
Dry weight | 0.098 | 0.269 | -0.432 | 0.626 | 0.3544 | |
Sex (M) | 0.016 | 0.423 | -0.814 | 0.849 | 0.4847 | |
Treatment (P) | -0.245 | 0.302 | -0.834 | 0.353 | 0.2049 | |
Sex (M) x Treatment (P) | -0.418 | 0.350 | -1.095 | 0.269 | 0.1189 | |
Chitin | ||||||
Dry weight | -0.483 | 0.263 | -1.001 | 0.030 | 0.0324 |
|
Sex (M) | 0.400 | 0.428 | -0.440 | 1.227 | 0.1722 | |
Treatment (P) | -0.115 | 0.283 | -0.667 | 0.456 | 0.3355 | |
Sex (M) x Treatment (P) | -0.316 | 0.327 | -0.953 | 0.324 | 0.1683 | |
Glycogen | ||||||
Dry weight | 0.334 | 0.266 | -0.187 | 0.854 | 0.1066 | |
Sex (M) | -0.270 | 0.423 | -1.094 | 0.560 | 0.2596 | |
Treatment (P) | 0.219 | 0.294 | -0.366 | 0.795 | 0.2241 | |
Sex (M) x Treatment (P) | 0.391 | 0.349 | -0.305 | 1.065 | 0.1340 | |
Lipids | ||||||
Dry weight | 0.543 | 0.255 | 0.041 | 1.041 | 0.0180 |
|
Sex (M) | -0.109 | 0.411 | -0.915 | 0.692 | 0.3932 | |
Treatment (P) | 0.388 | 0.273 | -0.157 | 0.916 | 0.0742 | |
Sex (M) x Treatment (P) | -0.052 | 0.308 | -0.640 | 0.557 | 0.4311 | |
Protein | ||||||
Dry weight | -0.216 | 0.267 | -0.743 | 0.301 | 0.2086 | |
Sex (M) | -0.019 | 0.428 | -0.860 | 0.808 | 0.4831 | |
Treatment (P) | -0.212 | 0.306 | -0.801 | 0.394 | 0.2456 | |
Sex (M) x Treatment (P) | 0.344 | 0.363 | -0.371 | 1.050 | 0.1706 | |
Dry weight | ||||||
Sex (M) | -1.613 | 0.141 | -1.892 | -1.341 | 0.0000 |
|
Treatment (P) | 0.528 | 0.159 | 0.217 | 0.839 | 0.0015 |
|
Sex (M) x Treatment (P) | -0.359 | 0.198 | -0.748 | 0.029 | 0.0354 |
|
summary.brmsfit()
sd(Lipid_Intercept)
) and slopes (e.g. sd(Dryweight_treatmentPolyandry)
), as well as the correlations between these effects (e.g. cor(Lipid_Intercept,Protein_Intercept)
is the correlation in line effects on lipids and proteins)Note that the model has converged (Rhat = 1) and the posterior is adequately samples (high ESS values).
brms_metabolite_SEM
Family: MV(gaussian, gaussian, gaussian, gaussian, gaussian, gaussian) Links: mu = identity; sigma = identity mu = identity; sigma = identity mu = identity; sigma = identity mu = identity; sigma = identity mu = identity; sigma = identity mu = identity; sigma = identity Formula: Lipid ~ sex * treatment + Dryweight + (treatment | p | line) Carbohydrate ~ sex * treatment + Dryweight + (treatment | p | line) Protein ~ sex * treatment + Dryweight + (treatment | p | line) Glycogen ~ sex * treatment + Dryweight + (treatment | p | line) Chitin ~ sex * treatment + Dryweight + (treatment | p | line) Dryweight ~ sex * treatment + (treatment | p | line) Data: scaled_metabolites %>% rename(Dryweight = Dry_weig (Number of observations: 48) Samples: 4 chains, each with iter = 5000; warmup = 2500; thin = 1; total post-warmup samples = 10000 Group-Level Effects: ~line (Number of levels: 8) Estimate Est.Error l-95% CI u-95% CI Rhat Bulk_ESS Tail_ESS sd(Lipid_Intercept) 0.09 0.15 0.00 0.52 1.00 2205 3122 sd(Lipid_treatmentPolyandry) 0.03 0.09 0.00 0.26 1.00 10416 5634 sd(Carbohydrate_Intercept) 0.07 0.14 0.00 0.49 1.00 4009 3563 sd(Carbohydrate_treatmentPolyandry) 0.05 0.14 0.00 0.47 1.00 6147 3091 sd(Protein_Intercept) 0.05 0.12 0.00 0.46 1.00 5474 3122 sd(Protein_treatmentPolyandry) 0.03 0.07 0.00 0.23 1.00 14351 6537 sd(Glycogen_Intercept) 0.03 0.07 0.00 0.23 1.00 11763 5625 sd(Glycogen_treatmentPolyandry) 0.03 0.06 0.00 0.17 1.00 17080 6554 sd(Chitin_Intercept) 0.07 0.13 0.00 0.45 1.00 4045 3642 sd(Chitin_treatmentPolyandry) 0.04 0.10 0.00 0.32 1.00 10529 5452 sd(Dryweight_Intercept) 0.05 0.07 0.00 0.26 1.00 3499 4233 sd(Dryweight_treatmentPolyandry) 0.03 0.05 0.00 0.18 1.00 9771 6085 cor(Lipid_Intercept,Lipid_treatmentPolyandry) 0.00 0.28 -0.53 0.53 1.00 21961 6563 cor(Lipid_Intercept,Carbohydrate_Intercept) 0.01 0.28 -0.53 0.54 1.00 21503 6928 cor(Lipid_treatmentPolyandry,Carbohydrate_Intercept) -0.00 0.28 -0.52 0.52 1.00 13932 7502 cor(Lipid_Intercept,Carbohydrate_treatmentPolyandry) 0.00 0.28 -0.53 0.53 1.00 21292 7123 cor(Lipid_treatmentPolyandry,Carbohydrate_treatmentPolyandry) 0.00 0.28 -0.54 0.54 1.00 16111 7114 cor(Carbohydrate_Intercept,Carbohydrate_treatmentPolyandry) -0.00 0.28 -0.53 0.52 1.00 11393 7217 cor(Lipid_Intercept,Protein_Intercept) 0.00 0.27 -0.53 0.52 1.00 19726 6371 cor(Lipid_treatmentPolyandry,Protein_Intercept) 0.00 0.27 -0.51 0.52 1.00 15406 7396 cor(Carbohydrate_Intercept,Protein_Intercept) -0.00 0.28 -0.54 0.53 1.00 12967 6678 cor(Carbohydrate_treatmentPolyandry,Protein_Intercept) -0.00 0.28 -0.53 0.53 1.00 11298 7158 cor(Lipid_Intercept,Protein_treatmentPolyandry) 0.00 0.28 -0.53 0.54 1.00 20488 7090 cor(Lipid_treatmentPolyandry,Protein_treatmentPolyandry) 0.00 0.28 -0.53 0.54 1.00 15638 6415 cor(Carbohydrate_Intercept,Protein_treatmentPolyandry) 0.00 0.27 -0.52 0.53 1.00 12822 7402 cor(Carbohydrate_treatmentPolyandry,Protein_treatmentPolyandry) 0.01 0.27 -0.51 0.54 1.00 9969 6797 cor(Protein_Intercept,Protein_treatmentPolyandry) -0.00 0.28 -0.55 0.54 1.00 9096 7764 cor(Lipid_Intercept,Glycogen_Intercept) 0.01 0.28 -0.53 0.54 1.00 20387 6844 cor(Lipid_treatmentPolyandry,Glycogen_Intercept) 0.00 0.27 -0.52 0.52 1.00 15710 7288 cor(Carbohydrate_Intercept,Glycogen_Intercept) 0.00 0.27 -0.52 0.53 1.00 12027 7551 cor(Carbohydrate_treatmentPolyandry,Glycogen_Intercept) -0.00 0.28 -0.53 0.52 1.00 10155 6478 cor(Protein_Intercept,Glycogen_Intercept) -0.00 0.27 -0.53 0.53 1.00 8457 7573 cor(Protein_treatmentPolyandry,Glycogen_Intercept) -0.00 0.28 -0.53 0.53 1.00 7939 7545 cor(Lipid_Intercept,Glycogen_treatmentPolyandry) -0.00 0.28 -0.53 0.53 1.00 24265 6764 cor(Lipid_treatmentPolyandry,Glycogen_treatmentPolyandry) -0.00 0.28 -0.54 0.53 1.00 15931 6498 cor(Carbohydrate_Intercept,Glycogen_treatmentPolyandry) -0.00 0.27 -0.53 0.52 1.00 12481 7007 cor(Carbohydrate_treatmentPolyandry,Glycogen_treatmentPolyandry) -0.00 0.28 -0.54 0.53 1.00 10235 7304 cor(Protein_Intercept,Glycogen_treatmentPolyandry) -0.00 0.28 -0.54 0.53 1.00 9399 6972 cor(Protein_treatmentPolyandry,Glycogen_treatmentPolyandry) 0.00 0.28 -0.54 0.54 1.00 7546 6992 cor(Glycogen_Intercept,Glycogen_treatmentPolyandry) 0.00 0.28 -0.54 0.54 1.00 5830 6824 cor(Lipid_Intercept,Chitin_Intercept) -0.00 0.27 -0.54 0.52 1.00 18378 7300 cor(Lipid_treatmentPolyandry,Chitin_Intercept) -0.00 0.28 -0.53 0.53 1.00 15157 7133 cor(Carbohydrate_Intercept,Chitin_Intercept) -0.00 0.28 -0.54 0.54 1.00 12651 7259 cor(Carbohydrate_treatmentPolyandry,Chitin_Intercept) -0.00 0.28 -0.53 0.54 1.00 9382 7490 cor(Protein_Intercept,Chitin_Intercept) -0.00 0.27 -0.52 0.52 1.00 8910 7562 cor(Protein_treatmentPolyandry,Chitin_Intercept) -0.01 0.28 -0.54 0.52 1.00 8730 7568 cor(Glycogen_Intercept,Chitin_Intercept) 0.00 0.28 -0.53 0.55 1.00 6749 7815 cor(Glycogen_treatmentPolyandry,Chitin_Intercept) -0.00 0.28 -0.53 0.54 1.00 6389 7418 cor(Lipid_Intercept,Chitin_treatmentPolyandry) -0.00 0.28 -0.53 0.52 1.00 19844 6699 cor(Lipid_treatmentPolyandry,Chitin_treatmentPolyandry) -0.00 0.28 -0.54 0.53 1.00 15244 6811 cor(Carbohydrate_Intercept,Chitin_treatmentPolyandry) -0.00 0.27 -0.53 0.54 1.00 12465 7063 cor(Carbohydrate_treatmentPolyandry,Chitin_treatmentPolyandry) -0.00 0.28 -0.54 0.53 1.00 10408 7174 cor(Protein_Intercept,Chitin_treatmentPolyandry) -0.00 0.28 -0.53 0.53 1.00 8816 7344 cor(Protein_treatmentPolyandry,Chitin_treatmentPolyandry) -0.00 0.28 -0.54 0.54 1.00 7606 6910 cor(Glycogen_Intercept,Chitin_treatmentPolyandry) -0.00 0.27 -0.52 0.52 1.00 6873 7088 cor(Glycogen_treatmentPolyandry,Chitin_treatmentPolyandry) 0.00 0.28 -0.53 0.54 1.00 5843 6996 cor(Chitin_Intercept,Chitin_treatmentPolyandry) 0.00 0.28 -0.52 0.53 1.00 6069 7815 cor(Lipid_Intercept,Dryweight_Intercept) -0.00 0.27 -0.53 0.52 1.00 18667 7391 cor(Lipid_treatmentPolyandry,Dryweight_Intercept) 0.00 0.28 -0.53 0.54 1.00 13660 7205 cor(Carbohydrate_Intercept,Dryweight_Intercept) 0.01 0.28 -0.53 0.53 1.00 12763 7849 cor(Carbohydrate_treatmentPolyandry,Dryweight_Intercept) 0.01 0.27 -0.52 0.53 1.00 10423 8523 cor(Protein_Intercept,Dryweight_Intercept) 0.00 0.28 -0.52 0.54 1.00 8603 7815 cor(Protein_treatmentPolyandry,Dryweight_Intercept) 0.01 0.27 -0.52 0.52 1.00 7465 7701 cor(Glycogen_Intercept,Dryweight_Intercept) -0.00 0.28 -0.54 0.54 1.00 7282 7419 cor(Glycogen_treatmentPolyandry,Dryweight_Intercept) -0.00 0.28 -0.54 0.53 1.00 6136 7728 cor(Chitin_Intercept,Dryweight_Intercept) -0.01 0.27 -0.54 0.52 1.00 5978 7957 cor(Chitin_treatmentPolyandry,Dryweight_Intercept) 0.00 0.28 -0.54 0.54 1.00 5792 7394 cor(Lipid_Intercept,Dryweight_treatmentPolyandry) 0.00 0.28 -0.53 0.54 1.00 22796 7188 cor(Lipid_treatmentPolyandry,Dryweight_treatmentPolyandry) -0.00 0.28 -0.53 0.53 1.00 16207 6282 cor(Carbohydrate_Intercept,Dryweight_treatmentPolyandry) 0.00 0.28 -0.54 0.54 1.00 12835 6715 cor(Carbohydrate_treatmentPolyandry,Dryweight_treatmentPolyandry) 0.00 0.28 -0.53 0.53 1.00 9358 7304 cor(Protein_Intercept,Dryweight_treatmentPolyandry) -0.00 0.28 -0.54 0.53 1.00 9625 7476 cor(Protein_treatmentPolyandry,Dryweight_treatmentPolyandry) -0.00 0.28 -0.53 0.53 1.00 7337 6920 cor(Glycogen_Intercept,Dryweight_treatmentPolyandry) -0.00 0.28 -0.54 0.52 1.00 6819 7728 cor(Glycogen_treatmentPolyandry,Dryweight_treatmentPolyandry) 0.00 0.28 -0.53 0.54 1.00 6067 6988 cor(Chitin_Intercept,Dryweight_treatmentPolyandry) -0.01 0.28 -0.54 0.51 1.00 5833 7200 cor(Chitin_treatmentPolyandry,Dryweight_treatmentPolyandry) -0.00 0.28 -0.54 0.54 1.00 5239 7139 cor(Dryweight_Intercept,Dryweight_treatmentPolyandry) -0.00 0.28 -0.54 0.53 1.00 5400 7475 Population-Level Effects: Estimate Est.Error l-95% CI u-95% CI Rhat Bulk_ESS Tail_ESS Lipid_Intercept -0.13 0.24 -0.60 0.36 1.00 10469 7864 Carbohydrate_Intercept 0.22 0.27 -0.32 0.76 1.00 13115 8654 Protein_Intercept 0.03 0.28 -0.52 0.57 1.00 13448 9004 Glycogen_Intercept -0.07 0.26 -0.59 0.44 1.00 13458 8253 Chitin_Intercept -0.06 0.25 -0.56 0.44 1.00 11535 8165 Dryweight_Intercept 0.63 0.11 0.42 0.85 1.00 9568 8052 Lipid_sexMale -0.11 0.41 -0.92 0.69 1.00 9335 7441 Lipid_treatmentPolyandry 0.39 0.27 -0.16 0.92 1.00 10103 8009 Lipid_Dryweight 0.54 0.26 0.04 1.04 1.00 8351 7680 Lipid_sexMale:treatmentPolyandry -0.05 0.31 -0.64 0.56 1.00 13230 8425 Carbohydrate_sexMale 0.02 0.42 -0.81 0.85 1.00 12437 8601 Carbohydrate_treatmentPolyandry -0.25 0.30 -0.83 0.35 1.00 12018 8871 Carbohydrate_Dryweight 0.10 0.27 -0.43 0.63 1.00 10119 7625 Carbohydrate_sexMale:treatmentPolyandry -0.42 0.35 -1.09 0.27 1.00 14229 8368 Protein_sexMale -0.02 0.43 -0.86 0.81 1.00 12360 7390 Protein_treatmentPolyandry -0.21 0.31 -0.80 0.39 1.00 14839 8231 Protein_Dryweight -0.22 0.27 -0.74 0.30 1.00 11135 8313 Protein_sexMale:treatmentPolyandry 0.34 0.36 -0.37 1.05 1.00 15653 8652 Glycogen_sexMale -0.27 0.42 -1.09 0.56 1.00 12139 7957 Glycogen_treatmentPolyandry 0.22 0.29 -0.37 0.79 1.00 13292 7366 Glycogen_Dryweight 0.33 0.27 -0.19 0.85 1.00 10481 8175 Glycogen_sexMale:treatmentPolyandry 0.39 0.35 -0.31 1.07 1.00 14732 7645 Chitin_sexMale 0.40 0.43 -0.44 1.23 1.00 10733 7764 Chitin_treatmentPolyandry -0.12 0.28 -0.67 0.46 1.00 11418 8230 Chitin_Dryweight -0.48 0.26 -1.00 0.03 1.00 9206 7424 Chitin_sexMale:treatmentPolyandry -0.32 0.33 -0.95 0.32 1.00 13831 8148 Dryweight_sexMale -1.61 0.14 -1.89 -1.34 1.00 11838 6854 Dryweight_treatmentPolyandry 0.53 0.16 0.22 0.84 1.00 10285 7734 Dryweight_sexMale:treatmentPolyandry -0.36 0.20 -0.75 0.03 1.00 11158 8445 Family Specific Parameters: Estimate Est.Error l-95% CI u-95% CI Rhat Bulk_ESS Tail_ESS sigma_Lipid 0.74 0.09 0.59 0.93 1.00 8507 7563 sigma_Carbohydrate 1.00 0.11 0.80 1.25 1.00 10276 7344 sigma_Protein 1.02 0.12 0.82 1.28 1.00 11893 7864 sigma_Glycogen 0.95 0.11 0.76 1.18 1.00 15966 7829 sigma_Chitin 0.84 0.10 0.67 1.06 1.00 9460 8187 sigma_Dryweight 0.36 0.04 0.29 0.46 1.00 10797 8042 Residual Correlations: Estimate Est.Error l-95% CI u-95% CI Rhat Bulk_ESS Tail_ESS rescor(Lipid,Carbohydrate) -0.33 0.14 -0.59 -0.03 1.00 7334 7461 rescor(Lipid,Protein) -0.06 0.15 -0.35 0.23 1.00 14149 7543 rescor(Carbohydrate,Protein) 0.04 0.14 -0.24 0.31 1.00 12497 8434 rescor(Lipid,Glycogen) 0.04 0.15 -0.26 0.33 1.00 8500 7024 rescor(Carbohydrate,Glycogen) -0.00 0.14 -0.28 0.28 1.00 13776 8306 rescor(Protein,Glycogen) -0.14 0.14 -0.40 0.15 1.00 10458 7699 rescor(Lipid,Chitin) -0.06 0.15 -0.36 0.24 1.00 11747 8231 rescor(Carbohydrate,Chitin) -0.42 0.13 -0.64 -0.15 1.00 11948 8547 rescor(Protein,Chitin) 0.07 0.15 -0.22 0.35 1.00 11094 8636 rescor(Glycogen,Chitin) -0.03 0.14 -0.32 0.25 1.00 11076 7900 rescor(Lipid,Dryweight) 0.16 0.18 -0.21 0.49 1.00 8099 8284 rescor(Carbohydrate,Dryweight) 0.00 0.18 -0.35 0.35 1.00 7164 8051 rescor(Protein,Dryweight) -0.04 0.17 -0.36 0.29 1.00 8687 8025 rescor(Glycogen,Dryweight) 0.01 0.17 -0.33 0.35 1.00 8311 7984 rescor(Chitin,Dryweight) 0.25 0.18 -0.11 0.57 1.00 6236 7132 Samples were drawn using sampling(NUTS). For each parameter, Bulk_ESS and Tail_ESS are effective sample size measures, and Rhat is the potential scale reduction factor on split chains (at convergence, Rhat = 1).
Here, we use the model to predict the mean concentration of each metabolite (in standard units) in each treatment and sex (averaged across the eight replicate selection lines). We then calculate the effect size of treatment by subtracting the (sex-specific) mean for the M treatment from the mean for the P treatment; thus a value of 1 would mean that the P treatment has a mean that is larger by 1 standard deviation. Thus, the y-axis in the following graphs essentially shows the posterior estimate of standardised effect size (Cohen’s d), from the model shown above.
Because the model contains dry weight as a mediator variable, we created these predictions two different ways, and display the answer for both using tabs in the following figures/tables. Firstly, we predicted the means controlling for differences in dry weight between sexes and treatments; this was done by deriving the predictions dry weight set to its global mean, for both sexes and treatments. Secondly, we derived predictions without controlling for dry weight. This was done by deriving the predictions with dry weight set to its average value for the appropriate treatment-sex combination.
By clicking the tabs and comparing, one can see that the estimates of the treatment effect hardly change when differences in dry weight are controlled for. This indicates that dry mass does not have an important role in mediating the effect of treatment on metabolite composition, even though body size differs between treatments. Thus, we conclude that the M vs P treatments caused metabolite composition to evolve, through mechanisms other than the evolution of dry weight.
new <- expand_grid(sex = c("Male", "Female"),
treatment = c("Monogamy", "Polyandry"),
Dryweight = NA, line = NA) %>%
mutate(type = 1:n())
levels <- c("Carbohydrate", "Chitin", "Glycogen", "Lipid", "Protein", "Dryweight")
# Estimate mean dry weight for each of the 4 sex/treatment combinations
evolved_mean_dryweights <- data.frame(
new[,1:2],
fitted(brms_metabolite_SEM, re_formula = NA,
newdata = new %>% select(-Dryweight),
summary = TRUE, resp = "Dryweight")) %>%
as_tibble()
# Find the mean dry weight for males and females (across treatments)
male_dryweight <- mean(evolved_mean_dryweights$Estimate[1:2])
female_dryweight <- mean(evolved_mean_dryweights$Estimate[3:4])
new_metabolites <- bind_rows(
expand_grid(sex = c("Male", "Female"),
treatment = c("Monogamy", "Polyandry"),
Dryweight = c(male_dryweight, female_dryweight), line = NA) %>%
filter(sex == "Male" & Dryweight == male_dryweight |
sex == "Female" & Dryweight == female_dryweight) %>%
mutate(type = 1:4),
evolved_mean_dryweights %>% select(sex, treatment, Dryweight = Estimate) %>%
mutate(line = NA, type = 5:8)
)
# Predict data from the SEM of metabolites...
# Because we use sum contrasts for "line" and line=NA in the new data,
# this function predicts at the global means across the 4 lines (see ?posterior_epred)
fitted_values <- posterior_epred(
brms_metabolite_SEM, newdata = new_metabolites, re_formula = NA,
summary = FALSE, resp = c("Carbohydrate", "Chitin", "Glycogen", "Lipid", "Protein")) %>%
reshape2::melt() %>% rename(draw = Var1, type = Var2, variable = Var3) %>%
as_tibble() %>%
left_join(new_metabolites, by = "type") %>%
select(draw, variable, value, sex, treatment, Dryweight) %>%
mutate(variable = factor(variable, levels))
treat_diff_standard_dryweight <- fitted_values %>%
filter(Dryweight %in% c(male_dryweight, female_dryweight)) %>%
spread(treatment, value) %>%
mutate(`Difference in means (Poly - Mono)` = Polyandry - Monogamy)
treat_diff_actual_dryweight <- fitted_values %>%
filter(!(Dryweight %in% c(male_dryweight, female_dryweight))) %>%
select(-Dryweight) %>%
spread(treatment, value) %>%
mutate(`Difference in means (Poly - Mono)` = Polyandry - Monogamy)
summary_dat1 <- treat_diff_standard_dryweight %>%
filter(variable != 'Dryweight') %>%
rename(x = `Difference in means (Poly - Mono)`) %>%
group_by(variable, sex) %>%
summarise(`Difference in means (Poly - Mono)` = median(x),
`Lower 95% CI` = quantile(x, probs = 0.025),
`Upper 95% CI` = quantile(x, probs = 0.975),
p = 1 - as.numeric(bayestestR::p_direction(x)),
` ` = ifelse(p < 0.05, "*", ""),
.groups = "drop")
summary_dat2 <- treat_diff_actual_dryweight %>%
filter(variable != 'Dryweight') %>%
rename(x = `Difference in means (Poly - Mono)`) %>%
group_by(variable, sex) %>%
summarise(`Difference in means (Poly - Mono)` = median(x),
`Lower 95% CI` = quantile(x, probs = 0.025),
`Upper 95% CI` = quantile(x, probs = 0.975),
p = 1 - as.numeric(bayestestR::p_direction(x)),
` ` = ifelse(p < 0.05, "*", ""),
.groups = "drop")
sampled_draws <- sample(unique(fitted_values$draw), 100)
ylims <- c(-2.3, 2.3)
treat_diff_actual_dryweight %>%
filter(variable != 'Dryweight') %>%
ggplot(aes(x = sex, y = `Difference in means (Poly - Mono)`,fill = sex)) +
geom_hline(yintercept = 0, linetype = 2) +
stat_halfeye() +
geom_line(data = treat_diff_actual_dryweight %>%
filter(draw %in% sampled_draws) %>%
filter(variable != 'Dryweight'),
alpha = 0.8, size = 0.12, colour = "black", aes(group = draw)) +
geom_point(data = summary_dat2, pch = 21, colour = "black", size = 3.1) +
scale_fill_brewer(palette = 'Pastel1', direction = 1, name = "") +
scale_colour_brewer(palette = 'Pastel1', direction = 1, name = "") +
facet_wrap( ~ variable, nrow = 1) +
theme_bw() +
theme(legend.position = 'none',
strip.background = element_blank(),
panel.grid.major.x = element_blank()) +
coord_cartesian(ylim = ylims) +
ylab("Difference in means between\nselection treatments (P - M)") + xlab("Sex")
treat_diff_standard_dryweight %>%
filter(variable != 'Dryweight') %>%
ggplot(aes(x = sex, y = `Difference in means (Poly - Mono)`,fill = sex)) +
geom_hline(yintercept = 0, linetype = 2) +
stat_halfeye() +
geom_line(data = treat_diff_standard_dryweight %>%
filter(draw %in% sampled_draws) %>%
filter(variable != 'Dryweight'),
alpha = 0.8, size = 0.12, colour = "black", aes(group = draw)) +
geom_point(data = summary_dat1, pch = 21, colour = "black", size = 3.1) +
scale_fill_brewer(palette = 'Pastel1', direction = 1, name = "") +
scale_colour_brewer(palette = 'Pastel1', direction = 1, name = "") +
facet_wrap( ~ variable, nrow = 1) +
theme_bw() +
theme(legend.position = 'none',
strip.background = element_blank(),
panel.grid.major.x = element_blank()) +
coord_cartesian(ylim = ylims) +
ylab("Difference in means between\nselection treatments (P - M)") + xlab("Sex")
Version | Author | Date |
---|---|---|
f7c88a2 | lukeholman | 2020-12-10 |
summary_dat1 %>%
kable(digits = 3) %>%
kable_styling(full_width = FALSE)
variable | sex | Difference in means (Poly - Mono) | Lower 95% CI | Upper 95% CI | p | |
---|---|---|---|---|---|---|
Carbohydrate | Female | -0.250 | -0.834 | 0.353 | 0.205 | |
Carbohydrate | Male | -0.668 | -1.326 | 0.036 | 0.031 |
|
Chitin | Female | -0.119 | -0.667 | 0.456 | 0.336 | |
Chitin | Male | -0.434 | -1.014 | 0.169 | 0.078 | |
Glycogen | Female | 0.220 | -0.366 | 0.795 | 0.224 | |
Glycogen | Male | 0.616 | -0.024 | 1.233 | 0.031 |
|
Lipid | Female | 0.390 | -0.157 | 0.916 | 0.074 | |
Lipid | Male | 0.342 | -0.241 | 0.872 | 0.111 | |
Protein | Female | -0.211 | -0.801 | 0.394 | 0.246 | |
Protein | Male | 0.132 | -0.562 | 0.826 | 0.347 |
summary_dat2 %>%
kable(digits = 3) %>%
kable_styling(full_width = FALSE)
variable | sex | Difference in means (Poly - Mono) | Lower 95% CI | Upper 95% CI | p | |
---|---|---|---|---|---|---|
Carbohydrate | Female | -0.195 | -0.752 | 0.380 | 0.247 | |
Carbohydrate | Male | -0.650 | -1.314 | 0.055 | 0.034 |
|
Chitin | Female | -0.369 | -0.878 | 0.157 | 0.078 | |
Chitin | Male | -0.515 | -1.101 | 0.089 | 0.047 |
|
Glycogen | Female | 0.397 | -0.156 | 0.924 | 0.077 | |
Glycogen | Male | 0.673 | 0.017 | 1.293 | 0.022 |
|
Lipid | Female | 0.681 | 0.172 | 1.153 | 0.006 |
|
Lipid | Male | 0.433 | -0.152 | 0.969 | 0.066 | |
Protein | Female | -0.331 | -0.887 | 0.264 | 0.132 | |
Protein | Male | 0.099 | -0.605 | 0.795 | 0.386 |
This section essentially examines the treatment \(\times\) sex interaction term, by calculating the difference in the effect size of the P/M treatment between sexes, for each of the five metabolites. We find no strong evidence for a treatment \(\times\) sex interaction, i.e. the treatment effects did not differ detectably between sexes. However, the effect of the Polyandry treatment on glycogen concentration appears to be marginally more positive in males than females (probability of direction = 92.5%, similar to a one-sided p-value of 0.075).
treatsex_interaction_data1 <- treat_diff_actual_dryweight %>%
select(draw, variable, sex, d = `Difference in means (Poly - Mono)`) %>%
arrange(draw, variable, sex) %>%
group_by(draw, variable) %>%
summarise(`Difference in effect size between sexes (male - female)` = d[2] - d[1],
.groups = "drop") # males - females
treatsex_interaction_data1 %>%
filter(variable != 'Dryweight') %>%
ggplot(aes(x = `Difference in effect size between sexes (male - female)`, y = 1, fill = stat(x < 0))) +
geom_vline(xintercept = 0, linetype = 2) +
stat_halfeyeh() +
facet_wrap( ~ variable) +
scale_fill_brewer(palette = 'Pastel2', direction = 1, name = "") +
theme_bw() +
theme(legend.position = 'none',
strip.background = element_blank()) +
ylab("Posterior density")
treatsex_interaction_data2 <- treat_diff_standard_dryweight %>%
select(draw, variable, sex, d = `Difference in means (Poly - Mono)`) %>%
arrange(draw, variable, sex) %>%
group_by(draw, variable) %>%
summarise(`Difference in effect size between sexes (male - female)` = d[2] - d[1],
.groups = "drop") # males - females
treatsex_interaction_data2 %>%
filter(variable != 'Dryweight') %>%
ggplot(aes(x = `Difference in effect size between sexes (male - female)`, y = 1, fill = stat(x < 0))) +
geom_vline(xintercept = 0, linetype = 2) +
stat_halfeyeh() +
facet_wrap( ~ variable) +
scale_fill_brewer(palette = 'Pastel2', direction = 1, name = "") +
theme_bw() +
theme(legend.position = 'none',
strip.background = element_blank()) +
ylab("Posterior density")
Version | Author | Date |
---|---|---|
f7c88a2 | lukeholman | 2020-12-10 |
treatsex_interaction_data1 %>%
filter(variable != 'Dryweight') %>%
rename(x = `Difference in effect size between sexes (male - female)`) %>%
group_by(variable) %>%
summarise(`Difference in effect size between sexes (male - female)` = median(x),
`Lower 95% CI` = quantile(x, probs = 0.025),
`Upper 95% CI` = quantile(x, probs = 0.975),
p = 1 - as.numeric(bayestestR::p_direction(x)),
` ` = ifelse(p < 0.05, "*", ""),
.groups = "drop") %>%
kable(digits=3) %>%
kable_styling(full_width = FALSE)
variable | Difference in effect size between sexes (male - female) | Lower 95% CI | Upper 95% CI | p | |
---|---|---|---|---|---|
Carbohydrate | -0.458 | -1.103 | 0.209 | 0.089 | |
Chitin | -0.143 | -0.744 | 0.469 | 0.326 | |
Glycogen | 0.276 | -0.390 | 0.922 | 0.208 | |
Lipid | -0.248 | -0.802 | 0.329 | 0.199 | |
Protein | 0.423 | -0.265 | 1.102 | 0.113 |
treatsex_interaction_data2 %>%
filter(variable != 'Dryweight') %>%
rename(x = `Difference in effect size between sexes (male - female)`) %>%
group_by(variable) %>%
summarise(`Difference in effect size between sexes (male - female)` = median(x),
`Lower 95% CI` = quantile(x, probs = 0.025),
`Upper 95% CI` = quantile(x, probs = 0.975),
p = 1 - as.numeric(bayestestR::p_direction(x)),
` ` = ifelse(p < 0.05, "*", ""),
.groups = "drop") %>%
kable(digits=3) %>%
kable_styling(full_width = FALSE)
variable | Difference in effect size between sexes (male - female) | Lower 95% CI | Upper 95% CI | p | |
---|---|---|---|---|---|
Carbohydrate | -0.422 | -1.095 | 0.269 | 0.119 | |
Chitin | -0.317 | -0.953 | 0.324 | 0.168 | |
Glycogen | 0.397 | -0.305 | 1.065 | 0.134 | |
Lipid | -0.054 | -0.640 | 0.557 | 0.431 | |
Protein | 0.344 | -0.371 | 1.050 | 0.171 |
sessionInfo()
R version 4.0.3 (2020-10-10) Platform: x86_64-apple-darwin17.0 (64-bit) Running under: macOS Catalina 10.15.4 Matrix products: default BLAS: /Library/Frameworks/R.framework/Versions/4.0/Resources/lib/libRblas.dylib LAPACK: /Library/Frameworks/R.framework/Versions/4.0/Resources/lib/libRlapack.dylib locale: [1] en_AU.UTF-8/en_AU.UTF-8/en_AU.UTF-8/C/en_AU.UTF-8/en_AU.UTF-8 attached base packages: [1] stats graphics grDevices utils datasets methods base other attached packages: [1] knitrhooks_0.0.4 knitr_1.30 kableExtra_1.1.0 DT_0.13 tidybayes_2.0.3 brms_2.14.4 Rcpp_1.0.4.6 ggridges_0.5.2 gridExtra_2.3 [10] GGally_1.5.0 forcats_0.5.0 stringr_1.4.0 dplyr_1.0.0 purrr_0.3.4 readr_1.3.1 tidyr_1.1.0 tibble_3.0.1 ggplot2_3.3.2 [19] tidyverse_1.3.0 workflowr_1.6.2 loaded via a namespace (and not attached): [1] readxl_1.3.1 backports_1.1.7 plyr_1.8.6 igraph_1.2.5 svUnit_1.0.3 splines_4.0.3 crosstalk_1.1.0.1 [8] TH.data_1.0-10 rstantools_2.1.1 inline_0.3.15 digest_0.6.25 htmltools_0.5.0 rsconnect_0.8.16 fansi_0.4.1 [15] magrittr_2.0.1 modelr_0.1.8 RcppParallel_5.0.1 matrixStats_0.56.0 xts_0.12-0 sandwich_2.5-1 prettyunits_1.1.1 [22] colorspace_1.4-1 blob_1.2.1 rvest_0.3.5 haven_2.3.1 xfun_0.19 callr_3.4.3 crayon_1.3.4 [29] jsonlite_1.7.0 lme4_1.1-23 survival_3.2-7 zoo_1.8-8 glue_1.4.2 gtable_0.3.0 emmeans_1.4.7 [36] webshot_0.5.2 V8_3.4.0 pkgbuild_1.0.8 rstan_2.21.2 abind_1.4-5 scales_1.1.1 mvtnorm_1.1-0 [43] DBI_1.1.0 miniUI_0.1.1.1 viridisLite_0.3.0 xtable_1.8-4 stats4_4.0.3 StanHeaders_2.21.0-3 htmlwidgets_1.5.1 [50] httr_1.4.1 DiagrammeR_1.0.6.1 threejs_0.3.3 arrayhelpers_1.1-0 RColorBrewer_1.1-2 ellipsis_0.3.1 farver_2.0.3 [57] pkgconfig_2.0.3 reshape_0.8.8 loo_2.3.1 dbplyr_1.4.4 labeling_0.3 tidyselect_1.1.0 rlang_0.4.6 [64] reshape2_1.4.4 later_1.0.0 visNetwork_2.0.9 munsell_0.5.0 cellranger_1.1.0 tools_4.0.3 cli_2.0.2 [71] generics_0.0.2 broom_0.5.6 evaluate_0.14 fastmap_1.0.1 yaml_2.2.1 processx_3.4.2 fs_1.4.1 [78] nlme_3.1-149 whisker_0.4 mime_0.9 projpred_2.0.2 xml2_1.3.2 compiler_4.0.3 bayesplot_1.7.2 [85] shinythemes_1.1.2 rstudioapi_0.11 gamm4_0.2-6 curl_4.3 reprex_0.3.0 statmod_1.4.34 stringi_1.5.3 [92] highr_0.8 ps_1.3.3 Brobdingnag_1.2-6 lattice_0.20-41 Matrix_1.2-18 nloptr_1.2.2.1 markdown_1.1 [99] shinyjs_1.1 vctrs_0.3.0 pillar_1.4.4 lifecycle_0.2.0 bridgesampling_1.0-0 estimability_1.3 insight_0.8.4 [106] httpuv_1.5.3.1 R6_2.4.1 promises_1.1.0 codetools_0.2-16 boot_1.3-25 colourpicker_1.0 MASS_7.3-53 [113] gtools_3.8.2 assertthat_0.2.1 rprojroot_1.3-2 withr_2.2.0 shinystan_2.5.0 multcomp_1.4-13 bayestestR_0.6.0 [120] mgcv_1.8-33 parallel_4.0.3 hms_0.5.3 grid_4.0.3 coda_0.19-3 minqa_1.2.4 rmarkdown_2.5 [127] git2r_0.27.1 shiny_1.4.0.2 lubridate_1.7.8 base64enc_0.1-3 dygraphs_1.1.1.6