This package can be installed from Bioconductor:
if (!requireNamespace("BiocManager", quietly = TRUE))
install.packages("BiocManager")
BiocManager::install("SpatialFeatureExperiment")
SpatialFeatureExperiment
(SFE) is a new S4 class built on top of SpatialExperiment
(SPE). SpatialFeatureExperiment
incorporates geometries and geometry operations with the sf
package. Examples of supported geometries are Visium spots represented with polygons corresponding to their size, cell or nuclei segmentation polygons, tissue boundary polygons, pathologist annotation of histological regions, and transcript spots of genes. Using sf
, SpatialFeatureExperiment
leverages the GEOS C++ libraries underlying sf
for geometry operations, including algorithms for for determining whether geometries intersect, finding intersection geometries, buffering geometries with margins, etc. A schematic of the SFE object is shown below:
Below is a list of SFE features that extend the SPE object:
colGeometries
are sf
data frames associated with the entities that correspond to columns of the gene count matrix, such as Visium spots or cells. The geometries in the sf
data frames can be Visium spot centroids, Visium spot polygons, or for datasets with single cell resolution, cell or nuclei segmentations. Multiple colGeometries
can be stored in the same SFE object, such as one for cell segmentation and another for nuclei segmentation. There can be non-spatial, attribute columns in a colGeometry
rather than colData
, because the sf
class allows users to specify how attributes relate to geometries, such as “constant”, “aggregate”, and “identity”. See the agr
argument of the st_sf
documentation.colGraphs
are spatial neighborhood graphs of cells or spots. The graphs have class listw
(spdep
package), and the colPairs
of SingleCellExperiment
was not used so no conversion is necessary to use the numerous spatial dependency functions from spdep
, such as those for Moran’s I, Geary’s C, Getis-Ord Gi*, LOSH, etc. Conversion is also not needed for other classical spatial statistics packages such as spatialreg
and adespatial
.rowGeometries
are similar to colGeometries
, but support entities that correspond to rows of the gene count matrix, such as genes. A potential use case is to store transcript spots for each gene in smFISH or in situ sequencing based datasets.rowGraphs
are similar to colGraphs
. A potential use case may be spatial colocalization of transcripts of different genes.annotGeometries
are sf
data frames associated with the dataset but not directly with the gene count matrix, such as tissue boundaries, histological regions, cell or nuclei segmentation in Visium datasets, and etc. These geometries are stored in this object to facilitate plotting and using sf
for operations such as to find the number of nuclei in each Visium spot and which histological regions each Visium spot intersects. Unlike colGeometries
and rowGeometries
, the number of rows in the sf
data frames in annotGeometries
is not constrained by the dimension of the gene count matrix and can be arbitrary.annotGraphs
are similar to colGraphs
and rowGraphs
, but are for entities not directly associated with the gene count matrix, such as spatial neighborhood graphs for nuclei in Visium datasets, or other objects like myofibers. These graphs are relevant to spdep
analyses of attributes of these geometries such as spatial autocorrelation in morphological metrics of myofibers and nuclei. With geometry operations with sf
, these attributes and results of analyses of these attributes (e.g. spatial regions defined by the attributes) may be related back to gene expression.localResults
are similar to reducedDims
in SingleCellExperiment
, but stores results from univariate and bivariate local spatial analysis results, such as from localmoran
, Getis-Ord Gi*, and local spatial heteroscedasticity (LOSH). Unlike in reducedDims
, for each type of results (type is the type of analysis such as Getis-Ord Gi*), each feature (e.g. gene) or pair of features for which the analysis is performed has its own results. The local spatial analyses can also be performed for attributes of colGeometries
and annotGeometries
in addition to gene expression and colData
. Results of multivariate spatial analysis such as MULTISPATI PCA can be stored in reducedDims
.library(SpatialFeatureExperiment)
#>
#> Attaching package: 'SpatialFeatureExperiment'
#> The following object is masked from 'package:base':
#>
#> scale
library(SpatialExperiment)
#> Loading required package: SingleCellExperiment
#> Loading required package: SummarizedExperiment
#> Loading required package: MatrixGenerics
#> Loading required package: matrixStats
#>
#> Attaching package: 'MatrixGenerics'
#> The following objects are masked from 'package:matrixStats':
#>
#> colAlls, colAnyNAs, colAnys, colAvgsPerRowSet, colCollapse,
#> colCounts, colCummaxs, colCummins, colCumprods, colCumsums,
#> colDiffs, colIQRDiffs, colIQRs, colLogSumExps, colMadDiffs,
#> colMads, colMaxs, colMeans2, colMedians, colMins, colOrderStats,
#> colProds, colQuantiles, colRanges, colRanks, colSdDiffs, colSds,
#> colSums2, colTabulates, colVarDiffs, colVars, colWeightedMads,
#> colWeightedMeans, colWeightedMedians, colWeightedSds,
#> colWeightedVars, rowAlls, rowAnyNAs, rowAnys, rowAvgsPerColSet,
#> rowCollapse, rowCounts, rowCummaxs, rowCummins, rowCumprods,
#> rowCumsums, rowDiffs, rowIQRDiffs, rowIQRs, rowLogSumExps,
#> rowMadDiffs, rowMads, rowMaxs, rowMeans2, rowMedians, rowMins,
#> rowOrderStats, rowProds, rowQuantiles, rowRanges, rowRanks,
#> rowSdDiffs, rowSds, rowSums2, rowTabulates, rowVarDiffs, rowVars,
#> rowWeightedMads, rowWeightedMeans, rowWeightedMedians,
#> rowWeightedSds, rowWeightedVars
#> Loading required package: GenomicRanges
#> Loading required package: stats4
#> Loading required package: BiocGenerics
#>
#> Attaching package: 'BiocGenerics'
#> The following object is masked from 'package:SpatialFeatureExperiment':
#>
#> saveRDS
#> The following objects are masked from 'package:stats':
#>
#> IQR, mad, sd, var, xtabs
#> The following objects are masked from 'package:base':
#>
#> Filter, Find, Map, Position, Reduce, anyDuplicated, aperm, append,
#> as.data.frame, basename, cbind, colnames, dirname, do.call,
#> duplicated, eval, evalq, get, grep, grepl, intersect, is.unsorted,
#> lapply, mapply, match, mget, order, paste, pmax, pmax.int, pmin,
#> pmin.int, rank, rbind, rownames, sapply, saveRDS, setdiff, table,
#> tapply, union, unique, unsplit, which.max, which.min
#> Loading required package: S4Vectors
#>
#> Attaching package: 'S4Vectors'
#> The following object is masked from 'package:utils':
#>
#> findMatches
#> The following objects are masked from 'package:base':
#>
#> I, expand.grid, unname
#> Loading required package: IRanges
#> Loading required package: GenomeInfoDb
#> Loading required package: Biobase
#> Welcome to Bioconductor
#>
#> Vignettes contain introductory material; view with
#> 'browseVignettes()'. To cite Bioconductor, see
#> 'citation("Biobase")', and for packages 'citation("pkgname")'.
#>
#> Attaching package: 'Biobase'
#> The following object is masked from 'package:MatrixGenerics':
#>
#> rowMedians
#> The following objects are masked from 'package:matrixStats':
#>
#> anyMissing, rowMedians
library(SFEData)
library(sf)
#> Linking to GEOS 3.12.1, GDAL 3.8.4, PROJ 9.4.0; sf_use_s2() is TRUE
library(Matrix)
#>
#> Attaching package: 'Matrix'
#> The following object is masked from 'package:S4Vectors':
#>
#> expand
library(RBioFormats)
#> BioFormats library version 7.3.0
# Example dataset
(sfe <- McKellarMuscleData(dataset = "small"))
#> see ?SFEData and browseVignettes('SFEData') for documentation
#> loading from cache
#> class: SpatialFeatureExperiment
#> dim: 15123 77
#> metadata(0):
#> assays(1): counts
#> rownames(15123): ENSMUSG00000025902 ENSMUSG00000096126 ...
#> ENSMUSG00000064368 ENSMUSG00000064370
#> rowData names(6): Ensembl symbol ... vars cv2
#> colnames(77): AAATTACCTATCGATG AACATATCAACTGGTG ... TTCTTTGGTCGCGACG
#> TTGATGTGTAGTCCCG
#> colData names(12): barcode col ... prop_mito in_tissue
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : imageX imageY
#> imgData names(1): sample_id
#>
#> unit: full_res_image_pixels
#> Geometries:
#> colGeometries: spotPoly (POLYGON)
#> annotGeometries: tissueBoundary (POLYGON), myofiber_full (GEOMETRY), myofiber_simplified (GEOMETRY), nuclei (POLYGON), nuclei_centroid (POINT)
#>
#> Graphs:
#> Vis5A:
User interfaces to get or set the geometries and spatial graphs emulate those of reducedDims
and row/colPairs
in SingleCellExperiment
. Column and row geometries also emulate reducedDims
in internal implementation, while annotation geometries and spatial graphs differ.
Column and row geometries can be get or set with the dimGeometries()
or dimGeometry()
function. The MARGIN
argument is as in the apply()
function: MARGIN = 1
means row, and MARGIN = 2
means column.
dimGeometry()
gets or sets one particular geometry by name of index.
# Get Visium spot polygons
(spots <- dimGeometry(sfe, "spotPoly", MARGIN = 2))
#> Simple feature collection with 77 features and 1 field
#> Geometry type: POLYGON
#> Dimension: XY
#> Bounding box: xmin: 5000 ymin: 13000 xmax: 7000 ymax: 15000
#> CRS: NA
#> First 10 features:
#> geometry sample_id
#> AAATTACCTATCGATG POLYGON ((6472.186 13875.23... Vis5A
#> AACATATCAACTGGTG POLYGON ((5778.291 13635.43... Vis5A
#> AAGATTGGCGGAACGT POLYGON ((7000 13809.84, 69... Vis5A
#> AAGGGACAGATTCTGT POLYGON ((6749.535 13874.64... Vis5A
#> AATATCGAGGGTTCTC POLYGON ((5500.941 13636.03... Vis5A
#> AATGATGATACGCTAT POLYGON ((6612.42 14598.82,... Vis5A
#> AATGATGCGACTCCTG POLYGON ((5501.981 14118.62... Vis5A
#> AATTCATAAGGGATCT POLYGON ((6889.769 14598.22... Vis5A
#> ACGAGTACGGATGCCC POLYGON ((5084.397 13395.63... Vis5A
#> ACGCTAGTGATACACT POLYGON ((5639.096 13394.44... Vis5A
plot(st_geometry(spots))
# Setter
dimGeometry(sfe, "foobar", MARGIN = 2) <- spots
dimGeometries()
gets or sets all geometry of the given margin.
# Getter, all geometries of one margin
(cgs <- dimGeometries(sfe, MARGIN = 2))
#> List of length 2
#> names(2): spotPoly foobar
# Setter, all geometries
dimGeometries(sfe, MARGIN = 2) <- cgs
dimGeometryNames()
gets or sets the names of the geometries
(cg_names <- dimGeometryNames(sfe, MARGIN = 2))
#> [1] "spotPoly" "foobar"
# Setter
dimGeometryNames(sfe, MARGIN = 2) <- cg_names
colGeometry(sfe, "spotPoly")
, colGeometries(sfe)
, and colGeometryNames(sfe)
are shorthands for dimGeometry(sfe, "spotPoly", MARGIN = 2)
, dimGeometries(sfe, MARGIN = 2)
, and dimGeometryNames(sfe, MARGIN = 2)
respectively. Similarly, rowGeometr*(sfe, ...)
is a shorthand of dimGeometr*(sfe, ..., MARGIN = 1)
.
There are shorthands for some specific column or row geometries. For example, spotPoly(sfe)
is equivalent to colGeometry(sfe, "spotPoly")
for Visium spot polygons, and txSpots(sfe)
is equivalent to rowGeometry(sfe, "txSpots")
for transcript spots in single molecule technologies.
# Getter
(spots <- spotPoly(sfe))
#> Simple feature collection with 77 features and 1 field
#> Geometry type: POLYGON
#> Dimension: XY
#> Bounding box: xmin: 5000 ymin: 13000 xmax: 7000 ymax: 15000
#> CRS: NA
#> First 10 features:
#> geometry sample_id
#> AAATTACCTATCGATG POLYGON ((6472.186 13875.23... Vis5A
#> AACATATCAACTGGTG POLYGON ((5778.291 13635.43... Vis5A
#> AAGATTGGCGGAACGT POLYGON ((7000 13809.84, 69... Vis5A
#> AAGGGACAGATTCTGT POLYGON ((6749.535 13874.64... Vis5A
#> AATATCGAGGGTTCTC POLYGON ((5500.941 13636.03... Vis5A
#> AATGATGATACGCTAT POLYGON ((6612.42 14598.82,... Vis5A
#> AATGATGCGACTCCTG POLYGON ((5501.981 14118.62... Vis5A
#> AATTCATAAGGGATCT POLYGON ((6889.769 14598.22... Vis5A
#> ACGAGTACGGATGCCC POLYGON ((5084.397 13395.63... Vis5A
#> ACGCTAGTGATACACT POLYGON ((5639.096 13394.44... Vis5A
# Setter
spotPoly(sfe) <- spots
Annotation geometries can be get or set with annotGeometries()
or annotGeometry()
. In column or row geometries, the number of rows of the sf
data frame (i.e. the number of geometries in the data frame) is constrained by the number of rows or columns of the gene count matrix respectively, because just like rowData
and colData
, each row of a rowGeometry
or colGeometry
sf
data frame must correspond to a row or column of the gene count matrix respectively. In contrast, an annotGeometry
sf
data frame can have any dimension, not constrained by the dimension of the gene count matrix. Similar to column and row geometries, annotation geometries have annotGeometry()
, annotGeometries()
, and annotGeometryNames()
getters and setters.
# Getter, by name or index
(tb <- annotGeometry(sfe, "tissueBoundary"))
#> Simple feature collection with 1 feature and 2 fields
#> Geometry type: POLYGON
#> Dimension: XY
#> Bounding box: xmin: 5094 ymin: 13000 xmax: 7000 ymax: 14969
#> CRS: NA
#> ID geometry sample_id
#> 7 7 POLYGON ((5094 13000, 5095 ... Vis5A
plot(st_geometry(tb))
# Setter, by name or index
annotGeometry(sfe, "tissueBoundary") <- tb
# Get all annoation geometries as named list
ags <- annotGeometries(sfe)
# Set all annotation geometries with a named list
annotGeometries(sfe) <- ags
# Get names of annotation geometries
(ag_names <- annotGeometryNames(sfe))
#> [1] "tissueBoundary" "myofiber_full" "myofiber_simplified"
#> [4] "nuclei" "nuclei_centroid"
# Set names
annotGeometryNames(sfe) <- ag_names
There are shorthands for specific annotation geometries. For example, tissueBoundary(sfe)
is equivalent to annotGeometry(sfe, "tissueBoundary")
. cellSeg()
(cell segmentation) and nucSeg()
(nuclei segmentation) would first query colGeometries
(for single cell, single molecule technologies, equivalent to colGeometry(sfe, "cellSeg")
or colGeometry(sfe, "nucSeg")
), and if not found, they will query annotGeometries
(for array capture and microdissection technologies, equivalent to annotGeometry(sfe, "cellSeg")
or annotGeometry(sfe, "nucSeg")
).
# Getter
(tb <- tissueBoundary(sfe))
#> Simple feature collection with 1 feature and 2 fields
#> Geometry type: POLYGON
#> Dimension: XY
#> Bounding box: xmin: 5094 ymin: 13000 xmax: 7000 ymax: 14969
#> CRS: NA
#> ID geometry sample_id
#> 7 7 POLYGON ((5094 13000, 5095 ... Vis5A
# Setter
tissueBoundary(sfe) <- tb
Column, row, and annotation spatial graphs can be get or set with spatialGraphs()
and spatialGraph()
functions. Similar to dimGeometr*
functions, spatialGraph*
functions have a MARGIN
argument. However, since internally, row and column geometries are implemented very differently from annotation geometries, while row, column, and annotation graphs are implemented the same way, for the spatialGraph*
functions, MARGIN = 1
means rows, MARGIN = 2
means columns, and MARGIN = 3
means annotation. Similar to dimGeometry*
functions, there are rowGraph*
, colGraph*
, and annotGraph*
getter and setter functions for each margin.
This package wraps functions in the spdep
package to find spatial neighborhood graphs. In this example, triangulation is used to find the spatial graph; many other methods are also supported, such as k nearest neighbors, distance based neighbors, and polygon contiguity.
(g <- findSpatialNeighbors(sfe, MARGIN = 2, method = "tri2nb"))
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 77
#> Number of nonzero links: 428
#> Percentage nonzero weights: 7.218755
#> Average number of links: 5.558442
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 77 5929 77 28.0096 309.4083
plot(g, coords = spatialCoords(sfe))
# Set graph by name
spatialGraph(sfe, "graph1", MARGIN = 2) <- g
# Or equivalently
colGraph(sfe, "graph1") <- g
# Get graph by name
g <- spatialGraph(sfe, "graph1", MARGIN = 2L)
# Or equivalently
g <- colGraph(sfe, "graph1")
g
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 77
#> Number of nonzero links: 428
#> Percentage nonzero weights: 7.218755
#> Average number of links: 5.558442
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 77 5929 77 28.0096 309.4083
For Visium, spatial neighborhood graph of the hexagonal grid can be found with the known locations of the barcodes.
colGraph(sfe, "visium") <- findVisiumGraph(sfe)
plot(colGraph(sfe, "visium"), coords = spatialCoords(sfe))
All graphs of the SFE object, or if specified, of the margin of interest, can be get or set with spatialGraphs()
and the margin specific wrappers.
colGraphs(sfe)
#> $col
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 77
#> Number of nonzero links: 428
#> Percentage nonzero weights: 7.218755
#> Average number of links: 5.558442
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 77 5929 77 28.0096 309.4083
Similar to dimGeometries()
, the graphs have spatialGraphNames()
getter and setter and the margin specific wrappers.
colGraphNames(sfe)
#> [1] "graph1" "visium"
Thus far, the example dataset used only has one sample. The SpatialExperiment
(SPE) object has a special column in colData
called sample_id
, so data from multiple tissue sections can coexist in the same SPE object for joint dimension reduction and clustering while keeping the spatial coordinates separate. It’s important to keep spatial coordinates of different tissue sections separate because first, the coordinates would only make sense within the same section, and second, the coordinates from different sections can have overlapping numeric values.
SFE inherits from SPE, and with geometries and spatial graphs, sample_id
is even more important. The geometry and graph getter and setter functions have a sample_id
argument, which is optional when only one sample is present in the SFE object. This argument is mandatory if multiple samples are present, and can be a character vector for multiple samples or “all” for all samples. Below are examples of using the getters and setters for multiple samples.
# Construct toy dataset with 2 samples
sfe1 <- McKellarMuscleData(dataset = "small")
#> see ?SFEData and browseVignettes('SFEData') for documentation
#> loading from cache
sfe2 <- McKellarMuscleData(dataset = "small2")
#> see ?SFEData and browseVignettes('SFEData') for documentation
#> loading from cache
spotPoly(sfe2)$sample_id <- "sample02"
(sfe_combined <- cbind(sfe1, sfe2))
#> class: SpatialFeatureExperiment
#> dim: 15123 149
#> metadata(0):
#> assays(1): counts
#> rownames(15123): ENSMUSG00000025902 ENSMUSG00000096126 ...
#> ENSMUSG00000064368 ENSMUSG00000064370
#> rowData names(6): Ensembl symbol ... vars cv2
#> colnames(149): AAATTACCTATCGATG AACATATCAACTGGTG ... TTCCTCGGACTAACCA
#> TTCTGACCGGGCTCAA
#> colData names(12): barcode col ... prop_mito in_tissue
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : imageX imageY
#> imgData names(1): sample_id
#>
#> unit: full_res_image_pixels
#> Geometries:
#> colGeometries: spotPoly (POLYGON)
#> annotGeometries: tissueBoundary (GEOMETRY), myofiber_full (GEOMETRY), myofiber_simplified (GEOMETRY), nuclei (POLYGON), nuclei_centroid (POINT)
#>
#> Graphs:
#> Vis5A:
#> sample02:
Use the sampleIDs
function to see the names of all samples
sampleIDs(sfe_combined)
#> [1] "Vis5A" "sample02"
# Only get the geometries for the second sample
(spots2 <- colGeometry(sfe_combined, "spotPoly", sample_id = "sample02"))
#> Simple feature collection with 72 features and 1 field
#> Geometry type: POLYGON
#> Dimension: XY
#> Bounding box: xmin: 6000 ymin: 7025.865 xmax: 8000 ymax: 9000
#> CRS: NA
#> First 10 features:
#> sample_id geometry
#> AACACACGCTCGCCGC sample02 POLYGON ((6597.869 7842.575...
#> AACCGCTAAGGGATGC sample02 POLYGON ((6724.811 9000, 67...
#> AACGCTGTTGCTGAAA sample02 POLYGON ((6457.635 7118.991...
#> AACGGACGTACGTATA sample02 POLYGON ((6737.064 8083.571...
#> AATAGAATCTGTTTCA sample02 POLYGON ((7570.153 8564.368...
#> ACAAATCGCACCGAAT sample02 POLYGON ((8000 7997.001, 79...
#> ACAATTGTGTCTCTTT sample02 POLYGON ((6043.169 7843.77,...
#> ACAGGCTTGCCCGACT sample02 POLYGON ((7428.88 7358.195,...
#> ACCAGTGCGGGAGACG sample02 POLYGON ((6460.753 8566.757...
#> ACCCTCCCTTGCTATT sample02 POLYGON ((7847.503 8563.771...
# Only set the geometries for the second sample
# Leaving geometries of the first sample intact
colGeometry(sfe_combined, "spotPoly", sample_id = "sample02") <- spots2
# Set graph only for the second sample
colGraph(sfe_combined, "foo", sample_id = "sample02") <-
findSpatialNeighbors(sfe_combined, sample_id = "sample02")
# Get graph only for the second sample
colGraph(sfe_combined, "foo", sample_id = "sample02")
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 72
#> Number of nonzero links: 406
#> Percentage nonzero weights: 7.83179
#> Average number of links: 5.638889
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 72 5184 72 25.82104 289.8299
# Set graph of the same name for both samples
# The graphs are computed separately for each sample
colGraphs(sfe_combined, sample_id = "all", name = "visium") <-
findVisiumGraph(sfe_combined, sample_id = "all")
# Get multiple graphs of the same name
colGraphs(sfe_combined, sample_id = "all", name = "visium")
#> $Vis5A
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 77
#> Number of nonzero links: 394
#> Percentage nonzero weights: 6.645303
#> Average number of links: 5.116883
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 77 5929 77 31.68056 311.7544
#>
#> $sample02
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 72
#> Number of nonzero links: 366
#> Percentage nonzero weights: 7.060185
#> Average number of links: 5.083333
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 72 5184 72 29.83889 291.5833
# Or just all graphs of the margin
colGraphs(sfe_combined, sample_id = "all")
#> $Vis5A
#> $Vis5A$visium
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 77
#> Number of nonzero links: 394
#> Percentage nonzero weights: 6.645303
#> Average number of links: 5.116883
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 77 5929 77 31.68056 311.7544
#>
#>
#> $sample02
#> $sample02$foo
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 72
#> Number of nonzero links: 406
#> Percentage nonzero weights: 7.83179
#> Average number of links: 5.638889
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 72 5184 72 25.82104 289.8299
#>
#> $sample02$visium
#> Characteristics of weights list object:
#> Neighbour list object:
#> Number of regions: 72
#> Number of nonzero links: 366
#> Percentage nonzero weights: 7.060185
#> Average number of links: 5.083333
#>
#> Weights style: W
#> Weights constants summary:
#> n nn S0 S1 S2
#> W 72 5184 72 29.83889 291.5833
Sample IDs can also be changed, with the changeSampleIDs()
function, with a named vector whose names are the old names and values are the new names.
sfe_combined <- changeSampleIDs(sfe, replacement = c(Vis5A = "foo", sample02 = "bar"))
sfe_combined
#> class: SpatialFeatureExperiment
#> dim: 15123 77
#> metadata(0):
#> assays(1): counts
#> rownames(15123): ENSMUSG00000025902 ENSMUSG00000096126 ...
#> ENSMUSG00000064368 ENSMUSG00000064370
#> rowData names(6): Ensembl symbol ... vars cv2
#> colnames(77): AAATTACCTATCGATG AACATATCAACTGGTG ... TTCTTTGGTCGCGACG
#> TTGATGTGTAGTCCCG
#> colData names(12): barcode col ... prop_mito in_tissue
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : imageX imageY
#> imgData names(1): sample_id
#>
#> unit: full_res_image_pixels
#> Geometries:
#> colGeometries: spotPoly (POLYGON), foobar (POLYGON)
#> annotGeometries: tissueBoundary (POLYGON), myofiber_full (GEOMETRY), myofiber_simplified (GEOMETRY), nuclei (POLYGON), nuclei_centroid (POINT)
#>
#> Graphs:
#> foo: col: graph1, visium
An SFE object can be constructed from scratch with the assay matrices and metadata. In this toy example, dgCMatrix
is used, but since SFE inherits from SingleCellExperiment (SCE), other types of arrays supported by SCE such as delayed arrays should also work.
# Visium barcode location from Space Ranger
data("visium_row_col")
coords1 <- visium_row_col[visium_row_col$col < 6 & visium_row_col$row < 6,]
coords1$row <- coords1$row * sqrt(3)
# Random toy sparse matrix
set.seed(29)
col_inds <- sample(1:13, 13)
row_inds <- sample(1:5, 13, replace = TRUE)
values <- sample(1:5, 13, replace = TRUE)
mat <- sparseMatrix(i = row_inds, j = col_inds, x = values)
colnames(mat) <- coords1$barcode
rownames(mat) <- sample(LETTERS, 5)
That should be sufficient to create an SPE object, and an SFE object, even though no sf
data frame was constructed for the geometries. The constructor behaves similarly to the SPE constructor. The centroid coordinates of the Visium spots in the toy example can be converted into spot polygons with the spotDiameter
argument. Spot diameter in pixels in full resolution image can be found in the scalefactors_json.json
file in Space Ranger output.
sfe3 <- SpatialFeatureExperiment(list(counts = mat), colData = coords1,
spatialCoordsNames = c("col", "row"),
spotDiameter = 0.7)
When colData
contains columns for the centroid coordinates, the spatialCoordsNames
argument specifies which columns in colData
are for the coordinates, in the same order as x, y, and z (if applicable). If the coordinates are not in colData
, they can be specified separately in the spatialCoords
argument:
sfe3 <- SpatialFeatureExperiment(list(counts = mat),
spatialCoords = as.matrix(coords1[, c("col", "row")]),
spotDiameter = 0.7)
More geometries and spatial graphs can be added after calling the constructor.
Geometries can also be supplied in the constructor.
# Convert regular data frame with coordinates to sf data frame
cg <- df2sf(coords1[,c("col", "row")], c("col", "row"), spotDiameter = 0.7)
rownames(cg) <- colnames(mat)
sfe3 <- SpatialFeatureExperiment(list(counts = mat), colGeometries = list(foo = cg))
Space Ranger output can be read in a similar manner as in SpatialExperiment
; the returned SFE object has the spotPoly
column geometry for the spot polygons. If the filtered matrix is read in, then a column graph called visium
will also be present, for the spatial neighborhood graph of the Visium spots on tissue. The graph is not computed if all spots are read in regardless of whether they are on tissue.
dir <- system.file("extdata", package = "SpatialFeatureExperiment")
sample_ids <- c("sample01", "sample02")
samples <- file.path(dir, sample_ids)
Inside the outs
directory:
list.files(file.path(samples[1], "outs"))
#> [1] "filtered_feature_bc_matrix" "spatial"
There should also be raw_feature_bc_matrix
though this toy example only has the filtered matrix.
Inside the matrix directory:
list.files(file.path(samples[1], "outs", "filtered_feature_bc_matrix"))
#> [1] "barcodes.tsv" "features.tsv" "matrix.mtx"
Inside the spatial
directory:
list.files(file.path(samples[1], "outs", "spatial"))
#> [1] "aligned_fiducials.jpg" "barcode_fluorescence_intensity.csv"
#> [3] "detected_tissue_image.jpg" "scalefactors_json.json"
#> [5] "spatial_enrichment.csv" "tissue_hires_image.png"
#> [7] "tissue_lowres_image.png" "tissue_positions.csv"
Not all Visium datasets have all the files here. The barcode_fluorescence_intensity.csv
file is only present for datasets with fluorescent imaging rather than bright field H&E.
(sfe3 <- read10xVisiumSFE(samples, sample_id = sample_ids, type = "sparse",
data = "filtered", images = "hires"))
#> >>> 10X Visium data will be loaded: outs
#> >>> Adding spatial neighborhood graph to sample01
#> >>> 10X Visium data will be loaded: outs
#> >>> Adding spatial neighborhood graph to sample02
#> class: SpatialFeatureExperiment
#> dim: 5 25
#> metadata(0):
#> assays(1): counts
#> rownames(5): ENSG00000014257 ENSG00000142515 ENSG00000263639
#> ENSG00000163810 ENSG00000149591
#> rowData names(14): symbol Feature.Type ...
#> Median.Normalized.Average.Counts_sample02
#> Barcodes.Detected.per.Feature_sample02
#> colnames(25): GTGGCGTGCACCAGAG-1 GGTCCCATAACATAGA-1 ...
#> TGCAATTTGGGCACGG-1 ATGCCAATCGCTCTGC-1
#> colData names(10): in_tissue array_row ... channel3_mean channel3_stdev
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : pxl_col_in_fullres pxl_row_in_fullres
#> imgData names(4): sample_id image_id data scaleFactor
#>
#> unit: full_res_image_pixel
#> Geometries:
#> colGeometries: spotPoly (POLYGON)
#>
#> Graphs:
#> sample01: col: visium
#> sample02: col: visium
The barcode_fluorescence_intensity.csv
file is read into colData
. The spatial_enrichment.csv
file contains Moran’s I and its p-values for each gene; it is read into rowData
.
Instead of pixels in the full resolution image, the Visium data can be read so the units are microns. Full resolution pixels is related to microns by the spacing between spots, which is known to be 100 microns. The unit can be set in the unit
argument; for now only “micron” and “full_res_image_pixel” are supported for Visium:
(sfe3 <- read10xVisiumSFE(samples, sample_id = sample_ids, type = "sparse",
data = "filtered", images = "hires", unit = "micron"))
#> >>> 10X Visium data will be loaded: outs
#> >>> Converting pixels to microns
#> >>> Adding spatial neighborhood graph to sample01
#> >>> 10X Visium data will be loaded: outs
#> >>> Converting pixels to microns
#> >>> Adding spatial neighborhood graph to sample02
#> class: SpatialFeatureExperiment
#> dim: 5 25
#> metadata(0):
#> assays(1): counts
#> rownames(5): ENSG00000014257 ENSG00000142515 ENSG00000263639
#> ENSG00000163810 ENSG00000149591
#> rowData names(14): symbol Feature.Type ...
#> Median.Normalized.Average.Counts_sample02
#> Barcodes.Detected.per.Feature_sample02
#> colnames(25): GTGGCGTGCACCAGAG-1 GGTCCCATAACATAGA-1 ...
#> TGCAATTTGGGCACGG-1 ATGCCAATCGCTCTGC-1
#> colData names(10): in_tissue array_row ... channel3_mean channel3_stdev
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : pxl_col_in_fullres pxl_row_in_fullres
#> imgData names(4): sample_id image_id data scaleFactor
#>
#> unit: micron
#> Geometries:
#> colGeometries: spotPoly (POLYGON)
#>
#> Graphs:
#> sample01: col: visium
#> sample02: col: visium
The unit of the SFE object can be checked:
unit(sfe3)
#> [1] "micron"
At present, this is merely a string and SFE doesn’t perform unit conversion.
Unlike in SpatialExperiment
, SFE reads the images as terra::SpatRaster
objects, so the images are not loaded into memory unless necessary. Also, with terra
, if a larger image is associated with the SFE object, it will not be fully loaded into memory when plotted; rather, it’s downsampled.
class(imgRaster(getImg(sfe3)))
#> [1] "SpatRaster"
#> attr(,"package")
#> [1] "terra"
The commercialized MERFISH from Vizgen has a standard output format, that can be read into SFE with readVizgen()
. Because the cell segmentation from each field of view (FOV) has a separate HDF5 file and a MERFISH dataset can have hundreds of FOVs, we strongly recommend reading the MERFISH output on a server with a large number of CPU cores. Alternatively, some but not all MERFISH datasets store cell segmentation in a parquet
file, which can be more easily read into R. This requires the installation of arrow
. Here we read a toy dataset which is the first FOV from a real dataset:
fp <- tempdir()
dir_use <- VizgenOutput(file_path = file.path(fp, "vizgen"))
#> see ?SFEData and browseVignettes('SFEData') for documentation
#> loading from cache
#> The downloaded files are in /tmp/RtmpnNF32A/vizgen/vizgen_cellbound
list.files(dir_use)
#> [1] "cell_boundaries" "cell_boundaries.parquet"
#> [3] "cell_by_gene.csv" "cell_metadata.csv"
#> [5] "detected_transcripts.csv" "images"
The optional add_molecules
argument can be set to TRUE
to read in the transcript spots
(sfe_mer <- readVizgen(dir_use, z = 3L, image = "PolyT", add_molecules = TRUE))
#> >>> 1 `.parquet` files exist:
#> /tmp/RtmpnNF32A/vizgen/vizgen_cellbound/cell_boundaries.parquet
#> >>> using -> /tmp/RtmpnNF32A/vizgen/vizgen_cellbound/cell_boundaries.parquet
#> >>> Cell segmentations are found in `.parquet` file
#> >>> Checking polygon validity
#> >>> Reading transcript coordinates
#> >>> Converting transcript spots to geometry
#> >>> Writing reformatted transcript spots to disk
#> class: SpatialFeatureExperiment
#> dim: 88 1058
#> metadata(0):
#> assays(1): counts
#> rownames(88): CD4 TLL1 ... Blank-38 Blank-39
#> rowData names(0):
#> colnames(1058): 112824700230101249 112824700230101252 ...
#> 112824700330100920 112824700330100974
#> colData names(11): fov volume ... solidity sample_id
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : center_x center_y
#> imgData names(4): sample_id image_id data scaleFactor
#>
#> unit: micron
#> Geometries:
#> colGeometries: centroids (POINT), cellSeg (POLYGON)
#> rowGeometries: txSpots (MULTIPOINT)
#>
#> Graphs:
#> sample01:
The unit is always in microns. To make it easier and faster to read the data next time, the processed cell segmentation geometries and transcript spots are written to the same directory where the data resides:
list.files(dir_use)
#> [1] "cell_boundaries" "cell_boundaries.parquet"
#> [3] "cell_by_gene.csv" "cell_metadata.csv"
#> [5] "detected_transcripts.csv" "detected_transcripts.parquet"
#> [7] "images"
SFE supports reading the output from Xenium Onboarding Analysis (XOA) v1 and v2 with the function readXenium()
. Especially for XOA v2, arrow
is strongly recommended. The cell and nuclei polygon vertices and transcript spot coordinates are in parquet
files Similar to readVizgen()
, readXenium()
makes sf
data frames from the vertices and transcript spots and saves them as GeoParquet files.
dir_use <- XeniumOutput("v2", file_path = file.path(fp, "xenium"))
#> see ?SFEData and browseVignettes('SFEData') for documentation
#> loading from cache
#> The downloaded files are in /tmp/RtmpnNF32A/xenium/xenium2
list.files(dir_use)
#> [1] "cell_boundaries.csv.gz" "cell_boundaries.parquet"
#> [3] "cell_feature_matrix.h5" "cells.csv.gz"
#> [5] "cells.parquet" "experiment.xenium"
#> [7] "morphology_focus" "nucleus_boundaries.csv.gz"
#> [9] "nucleus_boundaries.parquet" "transcripts.csv.gz"
#> [11] "transcripts.parquet"
# RBioFormats issue: https://github.com/aoles/RBioFormats/issues/42
try(sfe_xen <- readXenium(dir_use, add_molecules = TRUE))
#> >>> Must use gene symbols as row names when adding transcript spots.
#> >>> Cell segmentations are found in `.parquet` file(s)
#> >>> Reading cell and nucleus segmentations
#> >>> Making MULTIPOLYGON nuclei geometries
#> >>> Making POLYGON cell geometries
#> Sanity checks on cell segmentation polygons:
#> >>> ..found 132 cells with (nested) polygon lists
#> >>> ..applying filtering
#> >>> Checking polygon validity
#> >>> Saving geometries to parquet files
#> >>> Reading cell metadata -> `cells.parquet`
#> >>> Reading h5 gene count matrix
#> >>> filtering cellSeg geometries to match 6272 cells with counts > 0
#> >>> filtering nucSeg geometries to match 6158 cells with counts > 0
#> >>> Reading transcript coordinates
#> >>> Converting transcript spots to geometry
#> >>> Writing reformatted transcript spots to disk
#> >>> Total of 116 features/genes with no transcript detected or `min_phred` < 20 are removed from SFE object
#> >>> To keep all features -> set `min_phred = NULL`
(sfe_xen <- readXenium(dir_use, add_molecules = TRUE))
#> >>> Must use gene symbols as row names when adding transcript spots.
#> >>> Preprocessed sf segmentations found
#> >>> Reading cell and nucleus segmentations
#> >>> Reading cell metadata -> `cells.parquet`
#> >>> Reading h5 gene count matrix
#> >>> filtering cellSeg geometries to match 6272 cells with counts > 0
#> >>> filtering nucSeg geometries to match 6158 cells with counts > 0
#> >>> Reading transcript coordinates
#> >>> Total of 116 features/genes with no transcript detected or `min_phred` < 20 are removed from SFE object
#> >>> To keep all features -> set `min_phred = NULL`
#> class: SpatialFeatureExperiment
#> dim: 398 6272
#> metadata(1): Samples
#> assays(1): counts
#> rownames(398): ABCC11 ACE2 ... UnassignedCodeword_0488
#> UnassignedCodeword_0497
#> rowData names(3): ID Symbol Type
#> colnames(6272): abclkehb-1 abcnopgp-1 ... odmgoega-1 odmgojlc-1
#> colData names(9): transcript_counts control_probe_counts ...
#> nucleus_area sample_id
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : x_centroid y_centroid
#> imgData names(4): sample_id image_id data scaleFactor
#>
#> unit: micron
#> Geometries:
#> colGeometries: centroids (POINT), cellSeg (POLYGON), nucSeg (MULTIPOLYGON)
#> rowGeometries: txSpots (MULTIPOINT)
#>
#> Graphs:
#> sample01:
list.files(dir_use)
#> [1] "cell_boundaries.csv.gz" "cell_boundaries.parquet"
#> [3] "cell_boundaries_sf.parquet" "cell_feature_matrix.h5"
#> [5] "cells.csv.gz" "cells.parquet"
#> [7] "experiment.xenium" "morphology_focus"
#> [9] "nucleus_boundaries.csv.gz" "nucleus_boundaries.parquet"
#> [11] "nucleus_boundaries_sf.parquet" "transcripts.csv.gz"
#> [13] "transcripts.parquet" "tx_spots.parquet"
This is similar to readVizgen()
and readXenium()
, except that the output doesn’t come with images.
dir_use <- CosMXOutput(file_path = file.path(fp, "cosmx"))
#> see ?SFEData and browseVignettes('SFEData') for documentation
#> loading from cache
#> The downloaded files are in /tmp/RtmpnNF32A/cosmx/cosmx
list.files(dir_use)
#> [1] "Run5642_S3_Quarter-polygons.csv"
#> [2] "Run5642_S3_Quarter_exprMat_file.csv"
#> [3] "Run5642_S3_Quarter_metadata_file.csv"
#> [4] "Run5642_S3_Quarter_tx_file.csv"
(sfe_cosmx <- readCosMX(dir_use, add_molecules = TRUE))
#> >>> Constructing cell polygons
#> >>> Checking polygon validity
#> >>> Reading transcript coordinates
#> >>> Converting transcript spots to geometry
#> >>> Writing reformatted transcript spots to disk
#> class: SpatialFeatureExperiment
#> dim: 960 27
#> metadata(0):
#> assays(1): counts
#> rownames(960): Chrna4 Slc6a1 ... NegPrb9 NegPrb10
#> rowData names(0):
#> colnames(27): 367_1 368_1 ... 581_1 583_1
#> colData names(19): fov cell_ID ... Max.DAPI sample_id
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : CenterX_global_px CenterY_global_px
#> imgData names(0):
#>
#> unit: full_res_image_pixel
#> Geometries:
#> colGeometries: centroids (POINT), cellSeg (POLYGON)
#> rowGeometries: txSpots (MULTIPOINT)
#>
#> Graphs:
#> sample01:
list.files(dir_use)
#> [1] "Run5642_S3_Quarter-polygons.csv"
#> [2] "Run5642_S3_Quarter_exprMat_file.csv"
#> [3] "Run5642_S3_Quarter_metadata_file.csv"
#> [4] "Run5642_S3_Quarter_tx_file.csv"
#> [5] "cell_boundaries_sf.parquet"
#> [6] "tx_spots.parquet"
A read function for Visium HD is in progress. Contribution for Akoya, Molecular Cartography, and Curio Seeker are welcome. See the issues.
SpatialExperiment
SPE objects can be coerced into SFE objects. If column geometries or spot diameter are not specified, then a column geometry called “centroids” will be created.
spe <- read10xVisium(samples, sample_ids, type = "sparse", data = "filtered",
images = "hires", load = FALSE)
For the coercion, column names must not be duplicate.
colnames(spe) <- make.unique(colnames(spe), sep = "-")
rownames(spatialCoords(spe)) <- colnames(spe)
(sfe3 <- toSpatialFeatureExperiment(spe))
#> class: SpatialFeatureExperiment
#> dim: 5 25
#> metadata(0):
#> assays(1): counts
#> rownames(5): ENSG00000014257 ENSG00000142515 ENSG00000263639
#> ENSG00000163810 ENSG00000149591
#> rowData names(1): symbol
#> colnames(25): GTGGCGTGCACCAGAG-1 GGTCCCATAACATAGA-1 ...
#> TGCAATTTGGGCACGG-1 ATGCCAATCGCTCTGC-1
#> colData names(4): in_tissue array_row array_col sample_id
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : pxl_col_in_fullres pxl_row_in_fullres
#> imgData names(4): sample_id image_id data scaleFactor
#>
#> unit:
#> Geometries:
#> colGeometries: centroids (POINT)
#>
#> Graphs:
#> sample01:
#> sample02:
If images are present in the SPE object, they will be converted into SpatRaster
when the SPE object is converted into SFE. Plotting functions in the Voyager
package relies on SpatRaster
to plot the image behind the geometries.
Seurat
Seurat objects canbe coerced into SFE objects though coercion from SFE to Seurat is not yet implemented.
dir_extdata <- system.file("extdata", package = "SpatialFeatureExperiment")
obj_vis <- readRDS(file.path(dir_extdata, "seu_vis_toy.rds"))
sfe_conv_vis <-
toSpatialFeatureExperiment(x = obj_vis,
image_scalefactors = "lowres",
unit = "micron",
BPPARAM = BPPARAM)
#> >>> Seurat Assays found: RNA
#> >>> RNA -> will be used as 'Main Experiment'
#> >>> Seurat spatial object found: VisiumV1
#> >>> 'full_res_image_pixel' units will be used ->
#> ie 'imagerow' & 'imagecol' without scaling factors
#> >>> set `unit = 'micron'` to convert spot coordinates to micron space
#> >>> Generating `sf` geometries
#> Warning: Layer 'data' is empty
#> Warning: Layer 'scale.data' is empty
#>
#> >>> Creating `SFE` object -> sample01
#> >>> Converting pixels to microns
sfe_conv_vis
#> class: SpatialFeatureExperiment
#> dim: 5 12
#> metadata(0):
#> assays(1): counts
#> rownames(5): ACPP KLK3 MSMB TGM4 TAGLN
#> rowData names(0):
#> colnames(12): GTGGCGTGCACCAGAG-1 GGTCCCATAACATAGA-1 ...
#> CTTCCTGCATATTTAC-1 CAATATGTAGATTTAC-1
#> colData names(7): orig.ident nCount_RNA ... in_tissue sample_id
#> reducedDimNames(0):
#> mainExpName: RNA
#> altExpNames(0):
#> spatialCoords names(2) : X Y
#> imgData names(0):
#>
#> unit: micron
#> Geometries:
#> colGeometries: spotPoly (POLYGON)
#>
#> Graphs:
#> sample01:
SFE objects can be concatenated with cbind
, as was done just now to create a toy example with 2 samples.
sfe_combined <- cbind(sfe1, sfe2)
The SFE object can also be subsetted like a matrix, like an SCE object. More complexity arises when it comes to the spatial graphs. The drop
argument of the SFE method [
determines what to do with the spatial graphs. If drop = TRUE
, then all spatial graphs will be removed, since the graphs with nodes and edges that have been removed are no longer valid. If drop = FALSE
, which is the default, then the spatial graphs will be reconstructed with the remaining nodes after subsetting. Reconstruction would only work when the original graphs were constructed with findSpatialNeighbors
or findVisiumGraph
in this package, which records the method and parameters used to construct the graphs. If reconstruction fails, then a waning will be issued and the graphs removed.
(sfe_subset <- sfe[1:10, 1:10, drop = TRUE])
#> Warning in subset.nb(x = nb, subset = subset): subsetting caused increase in
#> subgraph count
#> Warning in subset.nb(x = nb, subset = subset): subsetting caused increase in
#> subgraph count
#> Warning in subset.listw(graphs_sub[[s]][[m]][[g]], j_sample): subsetting
#> created no-neighbour observations, zero.policy set TRUE
#> class: SpatialFeatureExperiment
#> dim: 10 10
#> metadata(0):
#> assays(1): counts
#> rownames(10): ENSMUSG00000025902 ENSMUSG00000096126 ...
#> ENSMUSG00000090031 ENSMUSG00000033740
#> rowData names(6): Ensembl symbol ... vars cv2
#> colnames(10): AAATTACCTATCGATG AACATATCAACTGGTG ... ACGAGTACGGATGCCC
#> ACGCTAGTGATACACT
#> colData names(12): barcode col ... prop_mito in_tissue
#> reducedDimNames(0):
#> mainExpName: NULL
#> altExpNames(0):
#> spatialCoords names(2) : imageX imageY
#> imgData names(1): sample_id
#>
#> unit: full_res_image_pixels
#> Geometries:
#> colGeometries: spotPoly (POLYGON), foobar (POLYGON)
#> annotGeometries: tissueBoundary (POLYGON), myofiber_full (GEOMETRY), myofiber_simplified (GEOMETRY), nuclei (POLYGON), nuclei_centroid (POINT)
#>
#> Graphs:
#> Vis5A: col: graph1, visium
# Will give warning because graph reconstruction fails
sfe_subset <- sfe[1:10, 1:10]
If images are present, then they will be cropped to the bounding box of the remaining geometries after subsetting.
Just like sf
data frames, SFE objects can be subsetted by a geometry and a predicate relating geometries. For example, if all Visium spots were read into an SFE object regardless of whether they are in tissue, and the tissueBoundary
annotation geometry is provided, then the tissue boundary geometry can be used to subset the SFE object to obtain a new SFE object with only spots on tissue. Loupe does not give the tissue boundary polygon; such polygon can be obtained by thresholding the H&E image and converting the mask into polygons with OpenCV or the terra
R package, or by manual annotation in QuPath or LabKit (the latter needs to be converted into polygon).
Use the crop
function to directly get the subsetted SFE object. When images are present, they are cropped by the bounding box of the cropped geometries.
# Before
plot(st_geometry(tissueBoundary(sfe)))
plot(spotPoly(sfe), col = "gray", add = TRUE)
sfe_in_tissue <- crop(sfe, y = tissueBoundary(sfe), colGeometryName = "spotPoly")
Note that for large datasets with many geometries, cropping can take a while to run.
# After
plot(st_geometry(tissueBoundary(sfe)))
plot(spotPoly(sfe_in_tissue), col = "gray", add = TRUE)
crop
can also be used in the conventional sense of cropping, i.e. specifying a bounding box.
sfe_cropped <- crop(sfe, y = c(xmin = 5500, xmax = 6500, ymin = 13500, ymax = 14500),
colGeometryName = "spotPoly", sample_id = "Vis5A")
The colGeometryName
is used to determine which columns in the gene count matrix to keep. All geometries in the SFE object will be subsetted so only portions intersecting y
or the bounding box are kept. Since the intersection operation can produce a mixture of geometry types, such as intersection of two polygons producing polygons, points, and lines, the geometry types of the sf
data frames after subsetting may be different from those of the originals.
The cropping is done independently for each sample_id
, and only on sample_id
s specified. Again, sample_id
is optional when there is only one sample in the SFE object.
Geometry predicates and operations can also be performed to return the results without subsetting an SFE object. For example, one may want a logical vector indicating whether each Visium spot intersects the tissue, or a numeric vector of how many nuclei there are in each Visium spot. Or get the intersections between each Visium spot and nuclei. Again, the geometry predicates and operations are performed independently for each sample, and the sample_id
argument is optional when there is only one sample.
# Get logical vector
colData(sfe)$in_tissue <- annotPred(sfe, colGeometryName = "spotPoly",
annotGeometryName = "tissueBoundary",
sample_id = "Vis5A")
# Get the number of nuclei per Visium spot
colData(sfe)$n_nuclei <- annotNPred(sfe, "spotPoly", annotGeometryName = "nuclei")
# Get geometries of intersections of Visium spots and myofibers
spot_intersections <- annotOp(sfe, colGeometryName = "spotPoly",
annotGeometryName = "myofiber_simplified")
Sometimes the spatial coordinates of different samples can take very different values. The values can be made more comparable by moving all tissues so the bottom left corner of the bounding box would be at the origin, which would facilitate plotting and comparison across samples with geom_sf
and facet_*
.
To find the bounding box of all geometries in each sample of an SFE object:
SpatialFeatureExperiment::bbox(sfe, sample_id = "Vis5A")
#> xmin ymin xmax ymax
#> 5000 13000 7000 15000
To move the coordinates:
sfe_moved <- removeEmptySpace(sfe, sample_id = "Vis5A")
The original bounding box before moving is stored within the SFE object, which can be read by dimGeometry
setters so newly added geometries can have coordinates moved as well; this behavior can be turned off with the optional argument translate = FALSE
in dimGeometry
setters.
When images are present, they might need to be flipped to align with the spots. SpatialExperiment
implements methods to rotate and mirror images, and SFE implements methods for SFE objects to transpose and mirror images (terra::rotate()
does NOT rotate the image in the conventional sense – rather it changes the longitudes and where the globe is cut to project to 2D just like cutting a world map at the Atlantic vs. the Pacific).
SpatialExperiment
represents images with S4 classes inheriting from the VirtualSpatialImage
virtual class. To be compatible with SPE, SFE uses SpatRasterImage
, which is a thin wrapper of SpatRaster
inheriting from the virtual class. Transformations can be applied to SpatRasterImage
, as well as SFE objects with sample and image IDs specified.
When an image is transposed, it is flipped about the line going from top left to bottom right:
img <- getImg(sfe3, image_id = "hires")
plot(imgRaster(img))
plot(transposeImg(img) |> imgRaster())
Arguments for the SFE method of mirrorImg()
differ from those of the SPE method, to match terra::flip()
:
plot(mirrorImg(img, direction = "vertical") |> imgRaster())
plot(mirrorImg(img, direction = "horizontal") |> imgRaster())
Here we apply the transformation to an SFE object, where the image specified by the sample and image IDs are transformed:
sfe3 <- mirrorImg(sfe3, sample_id = "sample01", image_id = "hires")
So far, transposeImg()
and mirrorImg()
only transform the image. But the entire SFE object, including all the geometries and images, can be transformed at once.
sfe_mirrored <- mirror(sfe_in_tissue)
sfe_transposed <- transpose(sfe_in_tissue)
par(mfrow = c(1, 3), mar = rep(1.5, 4))
plot(st_geometry(tissueBoundary(sfe_in_tissue)))
plot(spotPoly(sfe_in_tissue), col = "gray", add = TRUE)
plot(st_geometry(tissueBoundary(sfe_mirrored)))
plot(spotPoly(sfe_mirrored), col = "gray", add = TRUE)
plot(st_geometry(tissueBoundary(sfe_transposed)))
plot(spotPoly(sfe_transposed), col = "gray", add = TRUE)
Transforming the entire SFE object can be useful when the tissue has a orientation and a conventional direction of the orientation, such as rostral is conventionally at the top while caudal is at the bottom in coronal brain sections, while anterior is at the left and posterior is at the right in saggital brain sections, to make data conform to the convention.
These are the limitations of the current version of SFE:
sf
, which is designed for vector spatial data (specifying coordinates of points, lines, and polygons vertices), SFE only supports vector data for the geometries, and raster (like an image, with a value at each pixel) is not supported. Vector is chosen, as it is a more memory efficient way to represent cell and nuclei segmentation than a raster map.listw
objects so no conversion is necessary to use the well-established spatial statistical methods in the spdep
, spatialreg
, and adespatial
packages. However, igraph
implements many graph analysis methods, and conversion is required to use them. Whether future versions of SFE will stick to listw
depends on importance of methods that use spatial graphs in igraph
class.sf
for is for 2D data.spatstat
package may be relevant, such as in analyzing spatial distribution of nuclei or transcript spots. As spatstat
predates sf
by over a decade, spatstat
does not play very nicely with sf
. However, since analyses of nuclei and transcript spot localization don’t center on the gene count matrix, whether spatstat
analyses should be integrated into SFE (which is centered on the gene count matrix) is questionable.# Clean up
unlink(file.path(fp, "vizgen"), recursive = TRUE)
unlink(file.path(fp, "xenium"), recursive = TRUE)
unlink(file.path(fp, "cosmx"), recursive = TRUE)
sessionInfo()
#> R version 4.4.1 (2024-06-14)
#> Platform: x86_64-pc-linux-gnu
#> Running under: Ubuntu 24.04.1 LTS
#>
#> Matrix products: default
#> BLAS: /media/volume/teran2_disk/biocbuild/bbs-3.20-bioc/R/lib/libRblas.so
#> LAPACK: /usr/lib/x86_64-linux-gnu/lapack/liblapack.so.3.12.0
#>
#> locale:
#> [1] LC_CTYPE=en_US.UTF-8 LC_NUMERIC=C
#> [3] LC_TIME=en_GB LC_COLLATE=C
#> [5] LC_MONETARY=en_US.UTF-8 LC_MESSAGES=en_US.UTF-8
#> [7] LC_PAPER=en_US.UTF-8 LC_NAME=en_US.UTF-8
#> [9] LC_ADDRESS=en_US.UTF-8 LC_TELEPHONE=en_US.UTF-8
#> [11] LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=en_US.UTF-8
#>
#> time zone: America/New_York
#> tzcode source: system (glibc)
#>
#> attached base packages:
#> [1] stats4 stats graphics grDevices utils datasets methods
#> [8] base
#>
#> other attached packages:
#> [1] RBioFormats_1.6.0 Matrix_1.7-1
#> [3] sf_1.0-19 SFEData_1.8.0
#> [5] SpatialExperiment_1.16.0 SingleCellExperiment_1.28.0
#> [7] SummarizedExperiment_1.36.0 Biobase_2.66.0
#> [9] GenomicRanges_1.58.0 GenomeInfoDb_1.42.0
#> [11] IRanges_2.40.0 S4Vectors_0.44.0
#> [13] BiocGenerics_0.52.0 MatrixGenerics_1.18.0
#> [15] matrixStats_1.4.1 SpatialFeatureExperiment_1.8.1
#> [17] BiocStyle_2.34.0
#>
#> loaded via a namespace (and not attached):
#> [1] spatstat.sparse_3.1-0 bitops_1.0-9
#> [3] EBImage_4.48.0 httr_1.4.7
#> [5] RColorBrewer_1.1-3 tools_4.4.1
#> [7] sctransform_0.4.1 utf8_1.2.4
#> [9] R6_2.5.1 HDF5Array_1.34.0
#> [11] uwot_0.2.2 lazyeval_0.2.2
#> [13] rhdf5filters_1.18.0 withr_3.0.2
#> [15] sp_2.1-4 gridExtra_2.3
#> [17] progressr_0.15.0 cli_3.6.3
#> [19] spatstat.explore_3.3-3 fastDummies_1.7.4
#> [21] sass_0.4.9 Seurat_5.1.0
#> [23] spatstat.data_3.1-2 arrow_17.0.0.1
#> [25] proxy_0.4-27 ggridges_0.5.6
#> [27] pbapply_1.7-2 dbscan_1.2-0
#> [29] R.utils_2.12.3 parallelly_1.39.0
#> [31] limma_3.62.1 RSQLite_2.3.7
#> [33] generics_0.1.3 spatstat.random_3.3-2
#> [35] ica_1.0-3 spdep_1.3-6
#> [37] dplyr_1.1.4 fansi_1.0.6
#> [39] abind_1.4-8 R.methodsS3_1.8.2
#> [41] terra_1.7-83 lifecycle_1.0.4
#> [43] yaml_2.3.10 edgeR_4.4.0
#> [45] rhdf5_2.50.0 SparseArray_1.6.0
#> [47] BiocFileCache_2.14.0 Rtsne_0.17
#> [49] grid_4.4.1 blob_1.2.4
#> [51] promises_1.3.0 dqrng_0.4.1
#> [53] ExperimentHub_2.14.0 crayon_1.5.3
#> [55] miniUI_0.1.1.1 lattice_0.22-6
#> [57] beachmat_2.22.0 cowplot_1.1.3
#> [59] KEGGREST_1.46.0 magick_2.8.5
#> [61] zeallot_0.1.0 pillar_1.9.0
#> [63] knitr_1.49 rjson_0.2.23
#> [65] boot_1.3-31 future.apply_1.11.3
#> [67] sfarrow_0.4.1 codetools_0.2-20
#> [69] leiden_0.4.3.1 wk_0.9.4
#> [71] glue_1.8.0 spatstat.univar_3.1-1
#> [73] data.table_1.16.2 vctrs_0.6.5
#> [75] png_0.1-8 spam_2.11-0
#> [77] gtable_0.3.6 assertthat_0.2.1
#> [79] cachem_1.1.0 xfun_0.49
#> [81] S4Arrays_1.6.0 mime_0.12
#> [83] DropletUtils_1.26.0 survival_3.7-0
#> [85] sfheaders_0.4.4 rJava_1.0-11
#> [87] tinytex_0.54 units_0.8-5
#> [89] statmod_1.5.0 fitdistrplus_1.2-1
#> [91] ROCR_1.0-11 nlme_3.1-166
#> [93] bit64_4.5.2 filelock_1.0.3
#> [95] RcppAnnoy_0.0.22 bslib_0.8.0
#> [97] irlba_2.3.5.1 KernSmooth_2.23-24
#> [99] colorspace_2.1-1 spData_2.3.3
#> [101] DBI_1.2.3 tidyselect_1.2.1
#> [103] bit_4.5.0 compiler_4.4.1
#> [105] curl_6.0.0 BiocNeighbors_2.0.0
#> [107] xml2_1.3.6 DelayedArray_0.32.0
#> [109] plotly_4.10.4 bookdown_0.41
#> [111] scales_1.3.0 classInt_0.4-10
#> [113] lmtest_0.9-40 rappdirs_0.3.3
#> [115] goftest_1.2-3 tiff_0.1-12
#> [117] stringr_1.5.1 digest_0.6.37
#> [119] spatstat.utils_3.1-1 fftwtools_0.9-11
#> [121] rmarkdown_2.29 XVector_0.46.0
#> [123] htmltools_0.5.8.1 pkgconfig_2.0.3
#> [125] jpeg_0.1-10 sparseMatrixStats_1.18.0
#> [127] dbplyr_2.5.0 fastmap_1.2.0
#> [129] rlang_1.1.4 htmlwidgets_1.6.4
#> [131] UCSC.utils_1.2.0 shiny_1.9.1
#> [133] DelayedMatrixStats_1.28.0 farver_2.1.2
#> [135] jquerylib_0.1.4 zoo_1.8-12
#> [137] jsonlite_1.8.9 BiocParallel_1.40.0
#> [139] R.oo_1.27.0 RCurl_1.98-1.16
#> [141] magrittr_2.0.3 scuttle_1.16.0
#> [143] GenomeInfoDbData_1.2.13 s2_1.1.7
#> [145] dotCall64_1.2 patchwork_1.3.0
#> [147] Rhdf5lib_1.28.0 munsell_0.5.1
#> [149] Rcpp_1.0.13-1 reticulate_1.39.0
#> [151] stringi_1.8.4 zlibbioc_1.52.0
#> [153] MASS_7.3-61 AnnotationHub_3.14.0
#> [155] plyr_1.8.9 parallel_4.4.1
#> [157] listenv_0.9.1 ggrepel_0.9.6
#> [159] deldir_2.0-4 Biostrings_2.74.0
#> [161] splines_4.4.1 tensor_1.5
#> [163] locfit_1.5-9.10 igraph_2.1.1
#> [165] spatstat.geom_3.3-3 RcppHNSW_0.6.0
#> [167] reshape2_1.4.4 BiocVersion_3.20.0
#> [169] evaluate_1.0.1 SeuratObject_5.0.2
#> [171] BiocManager_1.30.25 httpuv_1.6.15
#> [173] polyclip_1.10-7 RANN_2.6.2
#> [175] tidyr_1.3.1 purrr_1.0.2
#> [177] future_1.34.0 scattermore_1.2
#> [179] ggplot2_3.5.1 xtable_1.8-4
#> [181] e1071_1.7-16 RSpectra_0.16-2
#> [183] later_1.3.2 viridisLite_0.4.2
#> [185] class_7.3-22 tibble_3.2.1
#> [187] memoise_2.0.1 AnnotationDbi_1.68.0
#> [189] cluster_2.1.6 globals_0.16.3