hospitals, remote points of care, or at

the doctor’s practice.

A concept comes alive

The idea for the high-throughput

‘cell sorter’ chip was developed

two years ago (see https://vimeo.

com/82078661 and figure2). R&D

manager Liesbet Lagae was awarded

a prestigious ERC-grant to further

develop the promising idea. And

imec scientists made the first building

blocks and integrated them in a chip

of 4cm x 2cm (figure3), with the

following process for a cell analysis:

A drop of blood is inserted into the

input channel

The cells move through a

microfluidic channel with a high speed

of a few meters per second

One by one, the cells pass over an

image sensor while they are

illuminated by a laser

Based on the holographic image on

the sensor, a powerful computation

chip reconstructs an image of each

individual cell

The cell is identified (a tumor cell,

bacteria ...)

If the cell is of a type that we want

to investigate, it is separated in a

distinct microfluidic channel. This is

done with the help of steam bubbles

generated with heating elements

In the different output channels,

the live cells are collected for further

examination

A smart combination of silicon

technology, lens free microscopy and

ultrasmall steam bubbles

The ‘cell sorter’ chip is fabricated in

silicontechnology,thesametechnology

also used to make computer and

memory chips. One of the advantages

is that all building blocks can be mass-

produced extremely compact and be

integrated in a cost-efficient way. This

cost advantage becomes even greater

if more, parallel sorting structures are

integrated on the chip.

For visualizing and identifying cells,

the cell sorter uses lens-free digital

holographic microscopy. A laser on top

of the microfluidic channel illuminates

the cells as they pass. An image

sensor placed under the channel

captures the interference pattern of

the laser light and the light that has

passed through the cells. With this

interference pattern, an image of

the cell can be reconstructed. The

image quality is comparable to that

of phase contrast microscopy. We

optimized this technology, improving

the resolution considerably by using

a light point source (which creates a

‘zoom’ effect).

Experiments with blood samples

have shown that this technique

allows to distinguish between three

major classes of white blood cells:

granulocytes,

monocytes,

and

lymphocytes. These types differ in

their size and granularity of the cell

contents. In the experiments, we

first looked at samples that contain

only one type of cell. This allowed to

optimize the classification algorithm.

Next, we analyzed a full blood sample,

with the results shown in figure 5.

These results are highly comparable

with those obtained with a clinical

hematology analyzer (figure 6), which

proves the validity of the lens-free

microscopy technique.

The microfluidic switch that we use

to separate the cells of various types

is based on small, starlike heating

elements (figure 7). Our prototype

contains 288 such elements, situated

Figure 1: ‘Cell sorter’ chip that identifies and sorts 3,000

cells per second

Figure 2: Concept of the high-throughput ‘cell

sorter’ chip

New-Tech Magazine Europe l 31