Sedimentation and Centrifugation
Sedimentation and Centrifugation
Sedimentation and Centrifugation
SEDIMENTATION
After completing this chapter, the reader should be able to do the following:
r Determine the velocity of a sedimenting particle and calculate sedimentation
times, equivalent times, and sedimentation coefficients in gravitational and
centrifugal fields.
185
Analysis begins with the equation of motion of a particle of radius a and density
having mass m=(4/ 3)a3 in an inertial field moving radially at a distance R from
the center of rotation (Figure 5.1)
Assuming the particle is spherical,
(5.2.1) m
dv
4
4
= FiR + FbR + FdR = a3 2 R a3 0 2 R 6 a
3
3
dt
Direction of movement
Particle of radius a
Center of rotation
FIGURE5.1 Particle moving radially under the influence of an inertial field at distance R from the
center of rotation.
Sedimentation // 187
2 a 2 ( 0 ) 2 R
9
commonly called the centrifuge equation. If particles are allowed to sediment only
in the presence of gravity, then the inertial acceleration is g=9.8 m/s2, and 2R in
Equation (5.2.2) is replaced by g. If, however, the particle is moving outwardly from
the center of rotation in a centrifuge, R is not constant and is related to the velocity
by v=dR/dt, which gives from Equation (5.2.2) after rearrangement,
(5.2.3)
2
2
dR 2 a ( 0 ) dt
=
9
R
R = R0
(5.2.5) ln
This is a useful equation that relates time to the distance traveled by the particle.
5.2.2 Sensitivities
Creeping flow occurs at Reynolds numbers less than about 0.1 [1]. Table 5.1 shows
the sedimentation velocities for important bioparticles and biomolecules calculated
from Equation (5.2.2) with 0=1.0 g/cm3, =0.01 g cm1 s1 (poise), and representative values of and a. The sedimentation velocity and Reynolds number results
shown in Table 5.1 for yeast cells and bacterial cells at gravitation acceleration can
be multiplied by a centrifuges centrifugal acceleration to give the corresponding
Bioparticle or
biomolecule
Yeast cell
Bacteria cell
Protein
Sedimentation
Radius, a ( m)
Density,
(g/cm3)
Dimensionless
acceleration
(G= 2R/g)
Sedimentation
velocity,
v (cm/h)
Reynolds
number, Re
2.5
0.5
0.005
1.1
1.1
1.3
1
1
104
0.5
0.02
0.06
7 106
6 108
2 109
Sedimentation // 189
TABLE5.2 Measured Values of the Density of Representative Cells,
Organelles, and Biomolecules
Density, (g/cm3)
Ref.
Escherichia coli
Bacillus subtilis
1.09a
1.12
2
3
Arthrobacter sp.
1.17
Saccharomyces pombe
1.09
Saccharomyces cerevisiae
1.11
Amoeba proteus
1.02
Murine B cells
1.06
1.06
Peroxisomes
1.26a
Mitochondria
1.20
Plasma membranes
1.15a
Proteins
1.30
Ribosomes
1.57a
5
5
DNA
RNA
a
1.68
2.00a
Average value.
0.01
0.05
0.95
0.79
0.10
0.20
0.61
0.35
to particles of any size in a polydisperse system, using the volume fraction for all the
particles in the calculation [7].
The magnitude of the hindered settling effect for spherical particles as a function
of the particle volume fraction can be seen in Table 5.3. Note that hindered settling
can be significant for particle concentrations of a few percent or greater.
5.3 METHODS FOR ANALYSIS OF SEDIMENTATION
where Q is the outflow rate due to pumping or gravity feed, V0 is the initial volume in
each cylinder, c1,0 is the initial concentration of solute in the mixed chamber, and c2
Salt
solution
Paddle
stirrer
Salt
solution
Magnetic stirrer
Sedimentation // 191
When a body force is applied, velocity through a viscous medium is usually proportional to the accelerating field (examples are electric, magnetic, and inertial). In the
case of sedimentation, the resulting constant, a property of both the particle and the
medium, is the sedimentation coefficient, which is definedas
(5.3.2)s
2 R
2 a 2 ( 0 )
9
which defines s in terms of only properties of the particle and the medium. This coefficient is usually expressed at 20C and under conditions (viscosity and density) of
pure wateras
s20,w (s )
The sedimentation coefficient is often expressed in svedberg units, where 1013
s = 1 svedberg unit (S), named after the inventor of the ultracentrifuge, Theodor
Svedberg.
EXAMPLE5.1
dR 1
dt 2 R
or
2 s dt =
dR
R
t=
R
ln
R0
2s
ln(5 / 4)
=
1h
3600 s
2
= 8.1 h
2R
g
where R is usually defined as the radius of the centrifuge bowl. Thus, this dimensionless unit is measured in gsmultiples of the earths gravitational acceleration.
Arough approximation of the difficulty of a given separation by centrifugation is the
product of the dimensionless acceleration and the time required for the separation.
This product is called the equivalent time for the separation, and is writtenas
(5.3.5) Equivalent time Gt =
2R
t
g
Sedimentation // 193
Typical values of equivalent time are as follows:0.3 106 s for eukaryotic cells,
9 106 s for protein precipitates, 18 106 s for bacteria, and 1100 106 s for
ribosomes [10].
The equivalent time for the centrifugation of cells or biological particles of
unknown sedimentation properties may be estimated in a laboratory centrifuge.
Samples are centrifuged for various times until a constant volume of packed cells is
reached. The equivalent time Gt is calculated as the product of the G for the particular centrifuge and the time required to reach constant packed-cell volume. Acentrifuge that has commonly been used for this determination is the Gyro-Tester (Alfa
Laval, Inc.).
One approach to scale-up of a centrifugal operation is to assume constant equivalent time:
(5.3.6) (Gt )1 = (Gt )2
EXAMPLE5.2
Scale-up Based on Equivalent Time If bacterial cell debris has Gt=54 106 s [10],
how large must the centrifuge bowl be, and what centrifuge speed is needed to effect
a full sedimentation in a reasonable amount of time?
SOLUTION
Assume that a reasonable amount of time is about 2 h.From Equation (5.3.5) for Gt,
we can estimate the centrifuge speed if we know the centrifuge bowl size and the
time of centrifuging. It is reasonable to have a centrifuge that is 10cm in diameter.
Solving Equation (5.3.5) for using these values gives
Gtg
=
Rt
1/ 2
54 106 s 9.81 2
s
=
0.05 m 2(3600) s
1/ 2
= 1213
rad 1 rev
60 s
This speed can be achieved in a production tubular bowl centrifuge (see later:
Table 5.5).
The more commonly used analysis in industry is sigma analysis, which uses the
operation constant to characterize a centrifuge into which feed flows at volumetric
flow rate Q. Since the engineer often needs to determine Q on scale-up, a convenient
relationshipis
(5.3.7)Q = { g }[ ]
( 0 )g
9
and represents the geometry and speed of the centrifuge, as derived in the discussion of individual centrifuges in the next section; can also be thought of as
the cross-sectional area equivalent of the centrifuge, with units of length squared.
Therefore, in Equation (5.3.7) the accolades {} indicate properties of the particle to
be separated and of the fluid in which separation is occurring, and the square brackets [] indicate properties of the centrifuge.
The sedimentation velocity at 1 g can be estimated directly by using Equation
(5.3.8) if relevant properties of the system are known, or it can be measured in the
laboratory. Combining Equations (5.3.8) and (5.2.5), we obtain
(5.3.9) =
g
R
g ln
R0
2t
The common types of production centrifuges are illustrated in Figure 5.3, and a
comparison of the advantages and disadvantages of the different centrifuge designs
is given in Table 5.4 [11]. In the tubular centrifuge, solids deposit on the wall of the
bowl, and feed continues until the bowl is almost full, at which time the operation
is stopped and the solids removed. This type of centrifuge works well for particles
of relatively low sedimentation coefficient that must be recovered, such as protein precipitates. The disk centrifuges have a relatively high sedimentation area
for their volume and allow for continuous or intermittent solids discharge; they
Sedimentation // 195
Solids
(a)
(b)
(c)
Solids
(d )
(e)
(f )
FIGURE 5.3 Common types of production centrifuges: (a) tubular bowl, (b) multichamber, (c)
disk, nozzle, (d) disk, intermittent discharge, (e) scroll, and (f) basket. Arrows indicate the path of
the liquid phase; dashed lines show where the solids accumulate.
have been successfully used for the centrifugation of cells and cell lysates, where
the entire process often must be contained to avoid the escape of aerosols. The
scroll (or decanter) and basket centrifuges are typically used for particles that sediment relatively rapidly and can be washed well as packed solids, such as antibiotic
crystals.
Of all the centrifuges, the tubular and the disk types are probably the most
likely to be found in a bioseparation process involving the recovery of a protein
produced by cells. The capabilities of tubular and disk centrifuges are given in
Table 5.5 [12]. Note that there is generally a reduction in the maximum g-force
(dimensionless acceleration) as the diameter of the bowl increases. The tubular
bowl and disk centrifuges are analyzed to develop the value that can be used in
scaleup.
5.4.1 Tubular Bowl Centrifuge
The tubular bowl centrifuge allows fluid to enter at one end of a rotating cylinder
and exit at the opposite end, while particles move toward the wall of the cylinder
and captured both at the wall and by a weir at the exit, as indicated in Figure 5.4.
The liquid enters the bowl through an opening in the center of the lower bowl
head. The liquid is pushed by centrifugal force toward the periphery of the rotating bowl. Clarified liquid overflows a ring weir in the upper bowl head, the radius
Advantages
Disadvantages
Tubular bowl
tubular bowl
(d) Bowl cooling possible
Disk centrifuge
eliminates foaming
(c) Bowl cooling possible
Scroll or decanter
centrifuge
Basket centrifuge
solids
Speed
(rpm)
Maximum dimensionless
acceleration (G), 2R/g
Throughput
(liters/min)
44
105
50,000
15,000
61,400
13,200
0.21.0
0.438
127
15,000
16,000
0.875
254
10,000
14,200
40150
discharge
406
6,250
8,850
100570
686
762
4,200
3,300
6,760
4,630
1501500
1501500
Type
Tubular bowl
Sedimentation // 197
Exit
Ring weir
R0
R1
Liquid
interface
R
z
Feed
of which establishes the depth of the pool of liquid around the periphery of the
rotating bowl.
As in most engineering calculations, we wish to determine the flow rate Q. The
equations of motion that give the trajectory of sedimented particles are, first, in the
radial direction from Equation (5.2.2)
(5.4.1)
dR 2 a 2 ( 0 ) 2 R
=
9
dt
dz Q
Q
= =
2
dt A ( R0 R12 )
where A is the cross-sectional area for liquid flow in the centrifuge. These equations
of motion are combined to give the trajectory equation
dR
dR
(5.4.3) dt =
dz dz
dt
Substituting Equations (5.4.1) and (5.4.2) into this ratio, integrating dR between R0
and R1, and integrating dz between 0 and L and solving for Q gives
2
2
2
2 a ( 0 ) L ( R0 R1 )
(5.4.4) Q =
9
R
ln 0
R1
2
In view of Equations (5.3.7) and (5.3.8), the first factor in Equation (5.4.4) can be multiplied by g while the second is divided by g to give, again, Equation (5.3.7) for analysis:
(5.4.5) Q = { g }[ ]
L ( R02 R12 ) 2
R
g ln 0
R1
In practice, one uses a benchtop centrifuge to determine vg and chooses a centrifuge with throughput in the desired range. The centrifuge manufacturer supplies
for the selected centrifuge, and the flow rate is determined from Equation (5.4.5).
Alternatively, if the flow rate is constrained by some other factor, a custom centrifuge
with a specific can be constructed. This is also true for the continuous disk-stack
centrifuge, which is the subject of the next section.
A tubular bowl centrifuge operates in the batch mode. The bowl begins spinning,
either dry or full of water, which will be displaced by the solids suspension. The solids suspension is fed from the bottom of the bowl, as previously described, typically
through a jet that sprays the suspension onto the wall of the bowl. If the bowl begins
empty, the suspension distributes rapidly up the length of the bowl in a thin film. As
the suspension is fed, the liquid layer grows from the wall toward the center of the
bowl, until the thickness of the liquid layer is equal to the weir at the top of the bowl.
At this point, clarified liquid begins to exit the centrifuge at the rate of the feed. The
residence time of fluid in the bowlis
(5.4.7) =
L ( R02 R12 )
Q
As solids build up on the wall of the bowl, the inner radius of the bowl is effectively
decreased, reducing the residence time in the bowl, but also reducing the sedimentation distance and the maximum sedimentation velocity [see Equation (5.2.2)].
Referring to Equation (5.4.6), it can be seen that decreases with time during tubular bowl operation, as R0 approaches R1. Therefore, in order to continue to capture
particles in the tubular bowl, the flow rate has to be decreased as operation proceeds.
Sedimentation // 199
Practically, this is not donethe centrifuge is fed until particles break through, and
then the operation is discontinued and the bowl emptied of solids. Typically, the solids occupy no more than 80% of the bowl volume.
There are now commercial tubular bowl centrifuges which have mechanical
means to discharge solids. This feature makes operation of the tubular bowl centrifuge
more convenient and likely reduces downtime. However, the centrifuge still has to be
stopped, solids discharged and then restarted, which reduces the efficiency overall.
Typically, tubular bowl centrifuges can concentrate solids to essentially 100%
wet weight, or the weight you would measure by centrifuging a sample in the laboratory and decanting the supernatant. The solids are not required to flow in order to
operate the equipment; in fact, a tight pellet is preferred. This is an advantage of a
tubular bowl centrifuge over a disk centrifuge.
EXAMPLE5.3
g =
2 a ( 0 ) g
=
9
2
m3
g
m 106 cm
9
.
81
m3
cm 3
s2
g
9 0.01
cm s
= 5.45 10 6 cm/s
For complete recovery of the cells, we can use Equation (5.4.6) to estimate :
R02
R12
R
g ln 0
R
1
rev 2 rad
min
rev
9.81
100 cm 60 s
m
ln (5 / 2)
2
min
m
s
= 2.01 106 cm 2
liter
60 s
liter
= 0.66
min
103 cm3 min
Liquid
discharge
Conical disk
channels
Light
liquid
Heavier
sediment
Bowl
Disk channels
entrance
FIGURE5.5 Cross-sectional diagram of a disk centrifuge, showing the path of the liquid flow and
the collection of solids at the periphery.
Sedimentation // 201
R1
R
R0
FIGURE 5.6 Diagram of the zone between two disks and the definition of variables for a disk
centrifuge.
velocity, and , the sedimentation velocity of the particles. The following assumptions simplify the analysis:
1. Typically, 0, the flow velocity, is much greater than .
2. v0=Q/A, where A decreases as particles move toward the center.
3. The fluid velocity 0 is a function of y and goes to zero at the surface of the
disks.
The equation of motion in the x directionis
(5.4.8)
dx
= 0 sin
dt
This is simplified by the assumption that 0 is much greater than sin . The average
value of 0, denoted < 0>, is given by the flow rate Q divided by the cross-sectional
area A perpendicular to the flow for n disks:
(5.4.9) = Q =
0
Q
n( 2 R l )
where the R is the radial distance from the center of rotation, which is varying, and
l is the spacing between disks, which is fixed. The local value of 0 can be found by
multiplying < 0> by a function f (y) that gives the velocity variation between the
disks:
(5.4.10) =
0
Q
f ( y)
n(2 R l )
Integrating
across the space between the disks gives the average value of
0:
0 ( y)dy =
(5.4.11) 0
l
Q
n (2 Rl )
f ( y)dy = 1
(5.4.12) 0
l
sin
in comparison to
0,
we
dx
Q
=
f ( y)
dt n (2 Rl )
2 a 2 ( 0 ) 2 R
dy
= cos =
cos
9
dt
where the centrifugal velocity is obtained from Equation (5.2.2). The slope of the
trajectory of particles moving between any pair of disks is determined by combining
the equations of motion in the x and y directions:
dy
4 n a 2 ( 0 ) 2 R 2 l cos
dy
(5.4.15) = dt =
9Qf ( y)
dx dx
dt
Since dx=dR/sin , Equation (5.4.15) can be rearranged to give
4 n a 2 ( 0 ) 2 R 2 cot
(5.4.16)Q f ( y)dy =
dR
l
For the boundary conditions of integration, we focus on the particles that are the
most difficult to capture:such a particle entering at y=0 and R=R0 would exit at
y=l and R=R1 (see Figure 5.6). After integration of Equation (5.4.16) and using
the result of Equation (5.4.12), the result can be rearranged after multiplying and
dividing by g to yield
2
2
3
3
2 a ( 0 )g 2 n ( R0 R1 )cot
= { g }[ ]
9
3g
(5.4.17)Q =
Sedimentation // 203
Therefore, in a sensitivity analysis it is seen that the factor depends on the cube
of the bowl radius, the cotangent of the disk acute angle, the number of disks in the
stack, and, as in the tubular centrifuge, the square of the rotor speed. The disk acute
angle made by the conical disks is typically between 35 and 50 [13].
There are three types of disk centrifuges, depending on the mode of discharging the solids. In the batch mode, solids accumulate at the periphery of the bowl
until the bowl is nearly full, which is evidenced by turbidity of the liquid flowing
out of the centrifuge. At this point, the centrifuge needs to be shut off and the solids removed manually. The solids content of the feed needs to be low (0 to 1vol.
%) in order that the downtime for solids removal does not become excessive. In
the semicontinuous mode, the bowl is opened intermittently to allow solids to discharge through ports at the periphery. The solids content of the feed can be in the
range of 0 to 10vol. % for the intermittent discharge, and the solids exiting can
be nonflowable. For continuous operation, nozzles are placed at the periphery of
the centrifuge, and the solids content of the feed is in the range of 6 to 25% vol.
%.The solids exiting from the nozzles are flowable. Nozzles are distributed around
the periphery of the centrifuge and typically range from 12 to 24, depend on the
size of the centrifuge [13].
The time between discharges in the semi-continuous mode of operation of a disk
centrifuge with volumetric feed rate Q can be estimated from [13]:
(5.4.18) t d =
Vs e
Q f
where Vs is the solids holdup volume of the bowl (which typically is 40 to 50% of
the entire bowl volume) and e and f are the volume fractions of solids in the exiting
sediment and feed, respectively.
5.5 ULTRACENTRIFUGATION
One of the most important uses of ultracentrifugation has been the determination of
molecular weights by the combined measurement of sedimentation and diffusion coefficientsthe sedimentation-diffusion molecular weight. Proteins are the most common macromolecular compounds that are homogeneous with respect to molecular
weight, and it is for these compounds that the sedimentation-diffusion method has
been mainly used. The molecular weights of proteins, as well as for viruses, obtained
by this method have been found to be in excellent agreement with those obtained by
other methods [15]. Today, protein and nucleic acid molecular weights are commonly
determined by mass spectroscopy, electrophoresis, or chromatography (see Chapter2).
The development of the dependence of molecular weight on the sedimentation
and diffusion coefficients starts with the equation of motion for a sedimenting molecule at steady state [Equation (5.2.1)], which can be written as follows:
2
(5.5.1) V ( 0 ) R 6 a = 0
6 a
(1 V 0 ) 2 R
1
=
kT 6 a
sRT
D (1 V 0 )
where M is the molecular weight and here R is the gas constant. The partial specific
volume V can be easily determined as the slope of a plot of the specific volume of
the solution versus the weight fraction of the substance (see, e.g., the determination
of M of chymotrypsinogen by Schwert [16]). For accurate determinations of M using
this method, it is necessary that s and D be extrapolated to zero concentration. The
diffusion coefficient of the macromolecule can be measured from concentration profiles at equilibrium during sedimentation with a density gradient, or more commonly,
in a separate procedure such as by the free-diffusion method [15].
Sedimentation // 205
After cells have been lysed or bioparticles have been dispersed, it is often useful to
hasten the subsequent sedimentation or filtration step by reversibly increasing the
size of the particles to be separated. To this end, flocculation is used, and it occurs as
the result of adding a suitable chemical called a flocculant or by the selection of
naturally flocculating cells for fermentation, as in the case of lager yeast. Flocculants
can act by forming interparticle molecular bridges between particles, in which
case the flocculants are usually polymers or oligomers; they can also act by reducing
the repulsive forces between cells, usually by reducing the strength of the electrostatic field (for details see Chapter3, Section 3.4).
Centrifugation is frequently used after the addition of a flocculant to uncleared
broth or cell lysates. While the resulting aggregates are often treated as Stokes spheres,
they are actually open structures in which internal convection may occur. Various
theories of sedimentation of flocs have therefore been proposed, in view of the importance of this motion in the water-processing (sewage treatment) industry [17].
Chapter3 introduces the subject of flocculation but not the collection of the
flocs that are produced. In process engineering, the sedimentation of flocs is
usually treated empirically. Nevertheless, a number of formal treatments of this
problem have been carried out. In the standard Equation (5.2.2) for the sedimentation of spheres, empirical adjustments for sedimentation velocity of flocs can
be made on the basis of the reduction of density by the void volume fraction
of the floc and the reduction of the drag force by the drag reduction factor ,
which is also a function of the void volume fraction and the floc radius a. The
resulting Stokes sedimentation velocity of spherical flocs composed of particles
of density is then
(5.6.1) =
2 a 2 (1 )( 0 ) 2 R
9( , a )
To estimate the drag force reduction due to liquid flow through the void volume
1/ 2
of the floc, a dimensionless, normalized diameter a / k f is defined, in which
kf is the permeability of the floc for the fluid in which it is settling. The drag force
reduction factor has been related to the void volume fraction and the floc radius by a
variety of closely related functions, the most widely used of which seems to be [18]:
tanh
2 2 1
(5.6.2)(, a ) =
tanh
2 2 + 3 1
The determination of requires knowing the floc permeability kf, which can be calculated by using the following form of the Carman-Kozeny equation:
(5.6.3)k f =
2
KS 2 (1 )2
where Kozenys constant K = 4.8 [19], and S is Carmans specific surface area,
defined as the area of nonporous materials exposed to the liquid per unit volume,
as determined from the geometry of the individual particles that form the aggregate.
In addition to the collective behavior of particles in flocs, particles do not behave
totally independently when they are suspended at high concentration, such as at the
outer rim of a centrifuge or the bottom of a settling tank.
5.7 SEDIMENTATION AT LOW ACCELERATIONS
At low g forces, the sedimentation rate slows down and can sometimes be similar to
the rate of transport by diffusion, which is not affected by inertial forces. Here, we
examine ways to compare sedimentation and diffusion rates. The case of isothermal
settling is evaluated, which can lead to exponential distributions of concentration as
a function of height for small particles. Inclined sedimentation and field-flow fractionation, two operations that separate suspended particles on the basis of inertial
motion at 1 g, are also described.
5.7.1 Diffusion, Brownian Motion
where <x2> is the mean square distance traveled by a particle having diffusion coefficient D in time t. Using the Stokes-Einstein equation [Equation (5.5.3)] for spherical particles of radius a undergoing Brownian movement in a fluid of viscosity , we
can relate the diffusion coefficient to the thermal energy kT as follows:
(5.7.2)D =
kT
6 a
Sedimentation // 207
If the temperature T does not change over the height h of an ensemble of particles,
then the mean kinetic energy, which is proportional to k T, of all particles is the same
at all heights. The potential energy of a particle of mass m is usually expressed as
mgh; but if the particles are subject to buoyant forces in the fluid, the potential energy
becomes V ( 0)gh for particle volume V. From the Boltzmann distribution rule,
the concentration of particles at height h at equilibrium is therefore
V ( 0 )gh
kT
(5.7.3)c(h) = c(0)exp
Pe =
(5.7.4)
D L
If Pe < 0.1, diffusion is dominant; and c(h) is approximately constant or distributed.
In this case, Equation (5.7.3) should be used. If Pe > 10, sedimentation dominates,
and the concentration will eventually be high at h=0 and 0 elsewhere.
5.7.4 Inclined Sedimentation
where is the angle of inclination of the plates from the vertical, and b, w, and L
are the height, width, and length of the rectangular settler, respectively (Figure 5.7).
Inclined settlers are designed so that the path to the completion of sedimentation of a particle is extremely short, only a few millimeters, before the sedimented
particles begin to be convected toward the underflow. If the particulate fraction is
desired, it can be batch concentrated by continuous recycle of the underflow back
to the tank while the overflow bleeds off the supernatant. By the use of appropriate
settings, governed and predicted by the foregoing equations, it is also possible to
remove small particles in the overflow while retaining larger ones in the underflow,
thereby effecting a binary particle classification by size [20].
An important application of inclined settlers is in the removal of unproductive or
parasitic cells from bioreactors or cell culture systems; this method was used to remove
nonviable hybridoma cells from a cell culture, which resulted in high viable cell concentrations and high monoclonal antibody productivity over a 2-week culture period [20].
Pump
b
Overflow, Qo
Sampling
Sampling
Feed
Qf
L
Inclined settler
Underflow,Qu
FIGURE5.7 Diagram of an inclined settler system indicating variables used in the mass balance
[Equation (5.7.5)] and volumetric clearing rate [Equation (5.7.7)].
Sedimentation // 209
Since inclined settlers can be scaled up directly by increasing the area for settling, they potentially could be used at larger than laboratory scale. These settlers
operate at much higher capacities than vertical settlers because cells need to settle
only a distance of order b (see Figure 5.7) in an inclined settler, compared with a
distance of order L in a vertical settler.
5.7.5 Field-Flow Fractionation
where R is the retention ratio, defined as the ratio of the particle velocity to the mean
fluid velocity, a is the particle radius, b is the channel height, and is the steric factor that determines the particle net velocity and is approximately equal to (1 + /a),
where is the distance between the particle and the accumulation wall, as noted in
Sample injection
(inflow)
Field
Fraction collection
(outflow)
Flow vectors
FFF
cha
umu nnel
latio
nw
all
Acc
(a)
Field
1
(b)
FIGURE5.8 (a) Exploded view of a field-flow fractionation (FFF) channel. The field is the driving
force for separation, expected to act differentially on particles of different types. The field could
be gravitational, electrical, thermal, adsorptive, or steric, to name a few. (b) The principle of steric
FFF. Larger particles protrude into the higher-velocity region of laminar flow, hence are carried
farther in a specific amount of time than their smaller counterparts.
Figure 5.8. This technique has been shown to separate two cell-sized latex populations having sphere diameters of 10 and 15 m, and also to separate white and red
blood cells [21].
5.8 CENTRIFUGAL ELUTRIATION
Centrifugal elutriation is similar to inclined sedimentation and field-flow fractionation in that sedimentation takes place in the presence of fluid flow. In centrifugal elutriation, also called counterstreaming centrifugation, the effective length of a
sedimentation path is greatly extended by continuously pumping a counterstreaming
fluid in the opposite direction to that of sedimentation. To accomplish this, elutriation rotors have been designed. Such rotors perform functions similar to those of
the tubular bowl and disk-stack centrifuges. The sample suspension is held in the
rotor chamber, and the particles remain there as long as the two opposing forces are
in balance. By incremental increases in the flow rate of the fluid or by decreases in
the centrifugal force, distinct populations of particles (including cells) with relatively
homogeneous sizes can be eluted out of the rotor sequentially. The objective of elutriation is thus to collect particles of a specified volume by modifying the velocity of
the eluent fluid or the angular velocity of the rotor [22]. Both these variables must be
controlled with extreme care if precision of separation is to be achieved. The volume
and radius of the largest particle that can escape against the counterflow and be collected in the effluent can be determined from the equation of motion for a spherical
particle in an inertial field [Equation (5.2.1)], using the velocity v0 for the eluting
fluid [22]:
0
9 2
R ( 0 )
(5.8.1) V =
3
3/ 2
1/ 2
2 R ( 0 )
(5.8.2) a =
where V and a are the volume and radius of the particle, respectively. The capacity
of centrifugal elutriation in the batch mode is about 108 particles of about 10 m
diameter.
5.9 SUMMARY
Sedimentation // 211
r Sedimentation, like filtration, is used in early stages in downstream bioprocessing mainly for liquidsolid separations. Particles can be separated at large scale
in continuous centrifuges, and macromolecules can be separated, either for
analysis or collection, at small scale by ultracentrifugation at very high speeds.
r The sedimentation velocity of a particle depends on the square of its radius a
and linearly on the difference between its density and that of the suspending
solvent 0:
2 a 2 ( 0 ) 2 R
9
where is angular velocity (rad/s), R is the distance of the particle from the
center of rotation, and is fluid viscosity. The term 2 R is the centrifugal
acceleration.
r Corrections related to sedimentation calculations are required when particle
concentrations are high enough to hinder settling. Functions of concentration
are available for this correction.
r The sedimentation coefficient s, a property of both the particle and the medium,
is defined as
s
2R
which leads to
s=
2 a 2 ( 0 )
9
2R
g
where
g =
r
r
r
2 a 2 ( 0 ) g
9
NOMENCLATURE
a
A
b
c
D
g
G
h
Fx
k
kf
K
m
M
Sedimentation // 213
n
n
N
l
L
L
Pe
Q
R
R
R
Re
s
S
t
td
T
c
g
V
V0
Vs
V
w
Greek Letters
1/ 2
normalized diameter of a floc (= a / k f ) (dimensionless)
steric factor in field-flow fractionation ( 1 + / a ) (dimensionless)
distance between particle and accumulation wall in field-flow fractionation (cm)
void fraction of particles in a floc (dimensionless)
centrifuge disk acute angle (Figure 5.6) (degrees)
angle of inclination of an inclined settler from vertical (degrees)
e
f
PROBLEMS
5.1 Sedimentation versus Filtration Four particulate materials, A, B, C, and D, are suspended in water (density=1.00 g/cm3) and have the properties given in Table P5.1.
Choose between sedimentation and filtration for the separation of the following pairs
of particles from one another in mixed suspensions in water. Explain your answer in
each case.
(a) Afrom B
(b) B from C
(c) C from D
TABLE P5.1
Particle name
Density (g/cm3)
Radius ( m)
A
B
1.05
1.05
10
12
C
D
1.01
1.04
50
25
5.2 Strategies for Product Separation Yeast cells (a=3 m) in a fermentor secrete a
low molecular weight product at a concentration that produces uniform rod-shaped
crystals 2 6 m at about 20 times the number concentration (particles/ml) as the
cells. Using concise statements, design two possible strategies that take advantage of
the particulate nature of the product to separate the product from the broth and from the
cells. What additional information about the product crystals would be useful?
5.3 Isopycnic Sedimentation You wish to capture 3 m particles in a linear density gradient having a density of 1.12 g/cm3 at the bottom and 1.00 at the top. You layer a thin
particle suspension on the top of the 6cm column of fluid with a viscosity of 1.0 cp and
allow particles to settle at 1 g.
(a) How long must you wait for the particles you want (density=1.07 g/cm3) to sediment to within 0.1cm of their isopycnic level? Is it possible to determine the time
required for particles to sediment to exactly their isopycnic level?
(b) If instead of 1 g you use a centrifuge running at 800 rpm, and the top of the fluid
is 5cm from the center of rotation, how long must you centrifuge for the particles
to move to within 0.1cm of their isopycnic level?
5.4 Time Required for Sedimentation by Gravity Acertain reagent is added to a suspension of cells 4 m in diameter. These cells have a density of 1.08 g/cm3, and they are
suspended in liquid with a density of 1.00 g/cm3 and viscosity of 1.0 cp. This reagent
causes about half of the cells to form fairly solid aggregates, all of which are 90 m
Sedimentation // 215
in diameter and have density midway between that of the liquid and the cells. How
much time is required for all the aggregates to sediment to within 1cm of the bottom
of a vessel filled with suspension that is 0.5 m high? Approximately what fraction of
the single cells would have sedimented to this depth in the same amount of time? How
much time is required for all the single cells to sediment to within 1cm of the bottom
of the vessel?
5.5 Time Required for Sedimentation in a Centrifuge Using the results of Problem
5.4, determine the diameter and speed of a centrifuge required to reduce the total sedimentation time for the aggregates by a factor of ten, assuming you will use containers
that are 20cm high in the centrifuge. Also assume that the center of rotation is 3cm
from the tops of the containers. How much time must the same centrifuge be operated
to also sediment all the single cells? For simplicity, assume a swinging-bucket type of
centrifuge, in which the axis of the cylindrical vessel is horizontal, hence parallel to the
direction of sedimentation.
5.6 Determination of Sigma for a New Pilot Scale Centrifuge You test a new pilot
scale centrifuge by doing a breakthrough experiment using yeast as test particles. The
yeast were previously found to sediment at 100 m/s in a laboratory centrifuge operated at an acceleration of 500 g. The breakthrough flow rate is found to be 10 liters/
min. What is the sigma ( ) of this new centrifuge?
5.7 Bench Scale Tests for a Tubular Bowl Centrifuge You can bench-test a tubular bowl separation by first characterizing the product in a test-tube centrifugation.
Without actually knowing the size and density of the particles in the suspension, derive
an expression for the angular velocity required to capture the solids at a given volumetric flow rate Q in terms of the geometry of the tubular bowl and the quantities you
would measure in the test tube centrifugation.
5.8 Recovery of E.coli in a Tubular Bowl Centrifuge You are using a tubular bowl
centrifuge to recover E.coli cells containing an important bioproduct from a fermentation broth. In a preliminary run you find that 50% of the cells are recovered at a flow
rate of 5 liters/min and rotation speed of 6000 rpm.
(a) To increase the yield to 95% using the same centrifuge, what must the flow rate be?
(b) How much does the sedimentation velocity change if you double the rotation
speed?
5.9 Scale-up of a Disk Centrifuge Based on Laboratory Data Determine the maximum flow rate for the clarification of a suspension of lysed Escherichia coli cells by
a plant scale disk centrifuge based on laboratory data. The plant centrifuge has a bowl
diameter of 25.4cm and capabilities shown in Table 5.5. For this centrifuge, you also
know that =42, R1=8cm, R0=20cm, and number of disks=100 (see Figure 5.6).
In a laboratory centrifuge, you determined that it took a minimum of 17 min to
clarify the cell lysate at 12,000 rpm. The top of the culture being centrifuged was
32mm from the center of rotation, and the top of the packed solids was 79mm from
the center of rotation after 17 min.
5.10 Determination of Molecular Weight by Ultracentrifugation A new biopharmaceutical X has been discovered. Only crude extracts are available, and the material
is known to be a macromolecule. You are given a preparative ultracentrifuge and asked
to estimate the molecular weight of the macromolecule. You then do two experiments.
In the first one, you set up a linear sucrose density gradient and layer a crude sample of
X on top of it, using a 5cm long centrifuge tube (completely filled) and centrifuge to
equilibrium for 3days (72 h) at 25,000 rpm. In the second experiment, you place the
sample in its dilute buffer (viscosity the same as water) directly into two of the same
plastic ultracentrifuge tubes and run the centrifuge for 24 h at 25,000 rpm, at which
time you stop and remove fractions from one of the two tubes. After an additional 72 h
at 25,000 rpm, you stop the centrifuge and remove fractions from the remaining tube.
In all three cases, you collect 20 fractions, and each fraction corresponds to a 2.5mm
layer, so fraction 1 came from the bottom of the tube and fraction 20 came from the top.
Assume that the top of each centrifuge tube is 3cm from the center of rotation.
1.2
1.1
12
16
20
1.0
40
Density (g/cm3)
The company biologist then takes the three sets of 20 fractions and tests them on cell
cultures. The biologist returns data to you in terms of biological activity units in each
fraction, on a scale that is known to be linear with product mass. You then plot the data
from the three centrifuge tubes (Figure P5.10).
40
24 + 72 h
24 h
12
Fraction number
Fraction number
(a)
(b)
16
20
FIGURE P5.10 Ultracentrifugation results. (a) First experiment:crude extract layered on the top of
a tube with a linear sucrose density gradient and centrifuged to equilibrium for 72 h.(b) Second
experiment:crude extract in its dilute buffer in each of two of the same plastic tubes with one tube
centrifuged for 24 h and the other tube for 72 h.Centrifuge speed 25,000 rpm. Fractions, each corresponding to a 2.5mm layer in the tube, are numbered from the bottom to the top of each tube.
(a) From the appropriate equations for ultracentrifugation, use the data to estimate
the molecular weight of product X. (Hint: Use widths of profiles to estimate
diffusivity.)
(b) Make a sketch of the method for collecting fractions.
(c) After you completed your material balance calculations on the tubes, which were
8mm in diameter, the biologist told you that each tube originally contained 20 units
of biological activity. Speculate about why the material balance did not close.
5.11 Isothermal Settling Based on the data in Table 5.1, estimate the reduced concentration profile, c(h)/c(0), for the isothermal settling at 1 g of a protein with a
sedimentation radius of 0.005 m at ambient temperature up to a height of 100cm.
Recalculate the profile for a protein with a sedimentation radius of 0.002 m. Also
calculate the molecular weight of each protein. Explain the meaning of the concentration profiles.
Sedimentation // 217
5.12 Cost of Centrifugation In a bioprocess for the production of foreveron (a hypothetical youth-giving protein made by Kindergen, Inc.), a centrifuge is used to remove the
cells from the culture broth. The centrifuge operates continuously at 20 kW and processes 20 liters of feed culture broth per hour, discharging a liquid supernatant phase
containing 92 vol% of the feed liquid and no cells. The cell paste output has a density
of 1.08 g/cm3. The feed is processed batchwise in 40 liters of feed per batch. It takes a
busy technician ($20/h) 15 min to start the feed flow and 15 min to collect each batch
and deliver the supernatant and sediment to the next steps. Kindergen paid $50,000 for
the centrifuge, which has a useful life of 10years, buys a service contract for $5000/
year, and replaces the rotor every year for $10,000. The centrifuge is used only for
foreveron processing at two batches per day, 300days a year.
Calculate the cost of the centrifugal processing per kilogram of cell paste produced.
What contributes the most to the cost of centrifuging?
5.13 Estimation of Flow Rate for Centrifugation of Yeast Cells Amaximum flow rate
of 50 liters/min was achieved for the centrifugation of bacteria cells in a tubular centrifuge. The cells were 2.0m in diameter and had a density of 1.08 g/cm3. The medium
had a density of 1.01 g/cm3 and viscosity of 1.2 cp.
It is desired to centrifuge yeast cells in this same centrifuge. The yeast cells have a
diameter of 5.0m and a density of 1.10 g/cm3. The medium has a density of 1.02
g/cm3 and a viscosity of 1.3 cp. Estimate the maximum flow rate that can be used to
centrifuge the yeast cells.
5.14 Determination of Sigma from Laboratory Data In a laboratory centrifuge, it was
found that it took 300 s to centrifuge cells at 2000 rpm to a constant height of packed
cells. The top of the cell suspension and the top of the packed cells were 5cm and 9cm,
respectively, from the center of rotation of the centrifuge. For processing these cells in
a tubular bowl centrifuge at a flow rate of 20 liters/min, what should the value of be?
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